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🧬 Circular Phylogenetic Tree Pipeline with Resistance Gene Heatmaps

Complete workflow for Figure S1 generation – suitable for homepage documentation

---

📋 Pipeline Overview

WGS Reads (100 isolates)
        │
        ▼
┌─────────────────────┐
│ 1. Species Clustering│
│ • E. coli (n=24)     │
│ • K. pneumoniae (n=22)│
│ • A. baumannii (n=30)│
│ • P. aeruginosa (n=25)│
└─────────────────────┘
        │
        ▼
┌─────────────────────┐
│ 2. Genome Annotation│
│ • Prokka v1.14.5    │
│ • TIGRFAMs HMM DB   │
│ • Output: *.gff     │
└─────────────────────┘
        │
        ▼
┌─────────────────────┐
│ 3. Pangenome Analysis│
│ • Roary v3.13.0     │
│ • Core gene alignment│
│ • Gene P/A matrix   │
└─────────────────────┘
        │
        ▼
┌─────────────────────┐
│ 4. Resistance Gene  │
│    Detection        │
│ • Abricate + ResFinder│
│ • 13 β-lactamase genes│
└─────────────────────┘
        │
        ▼
┌─────────────────────┐
│ 5. Phylogenetic Tree│
│ • RAxML-NG          │
│ • GTR+G model       │
│ • 1000 bootstraps   │
└─────────────────────┘
        │
        ▼
┌─────────────────────┐
│ 6. Visualization    │
│ • ggtree (R)        │
│ • Circular layout   │
│ • ST-colored tips   │
│ • Gene heatmap ring │
└─────────────────────┘

---

🔧 Step-by-Step Commands

1️⃣ Prokka Annotation (per species)

#!/bin/bash
# prokka_run.sh

SPECIES_CONFIG=(
    "ecoli:Escherichia:coli"
    "kpneumoniae:Klebsiella:pneumoniae"
    "abaumannii:Acinetobacter:baumannii"
    "paeruginosa:Pseudomonas:aeruginosa"
)

for config in "${SPECIES_CONFIG[@]}"; do
    IFS=':' read -r SPECIES_KEY GENUS SPECIES_NAME <<< "$config"

    for SAMPLE in $(cat samples_${SPECIES_KEY}.txt); do
        prokka --force \
            --outdir prokka/${SPECIES_KEY}/${SAMPLE} \
            --cpus 8 \
            --kingdom Bacteria \
            --genus "${GENUS}" \
            --species "${SPECIES_NAME}" \
            --addgenes --addmrna \
            --prefix "${SAMPLE}" \
            --locustag "${SAMPLE}" \
            --hmm /media/jhuang/Titisee/GAMOLA2/TIGRfam_db/TIGRFAMs_15.0_HMM.LIB \
            assemblies/${SAMPLE}.fasta
    done
done

2️⃣ Roary Pangenome Analysis

#!/bin/bash
# roary_run.sh

# A. baumannii
roary -f roary/abaumannii -e --mafft -p 40 \
    prokka/abaumannii/*/*.gff

# E. coli
roary -f roary/ecoli -e --mafft -p 40 \
    prokka/ecoli/*/*.gff

# K. pneumoniae
roary -f roary/kpneumoniae -e --mafft -p 40 \
    prokka/kpneumoniae/*/*.gff

# P. aeruginosa
roary -f roary/paeruginosa -e --mafft -p 40 \
    prokka/paeruginosa/*/*.gff

3️⃣ Resistance Gene Detection (Abricate + ResFinder)

#!/bin/bash
# abricate_run.sh

# Setup databases (one-time)
abricate --setupdb

# Define target genes
TARGET_GENES="blaCTX-M,blaIMP,blaKPC,blaNDM-1,blaNDM-5,blaOXA-23-like,blaOXA-24-like,blaOXA-48-like,blaOXA-58-like,blaPER-1,blaSHV,blaVEB-1,blaVIM"

for SPECIES in ecoli kpneumoniae abaumannii paeruginosa; do
    for SAMPLE in $(cat samples_${SPECIES}.txt); do
        # Run against ResFinder
        abricate --db resfinder \
            --minid 90 --mincov 80 \
            assemblies/${SAMPLE}.fasta \
            > abricate/${SPECIES}/${SAMPLE}.resfinder.tsv

        # Extract target genes to CSV-ready format
        awk -F'\t' -v sample="${SAMPLE}" '
            NR==1 {next}
            $10 ~ /blaCTX-M|blaIMP|blaKPC|blaNDM-1|blaNDM-5|blaOXA-23-like|blaOXA-24-like|blaOXA-48-like|blaOXA-58-like|blaPER-1|blaSHV|blaVEB-1|blaVIM/ {
                gene=$10; gsub(/[^a-zA-Z0-9.-]/,"_",gene);
                print sample"\t"gene"\t+"
            }' abricate/${SPECIES}/${SAMPLE}.resfinder.tsv
    done | pivot to wide format > isolate_${SPECIES}.csv
done

4️⃣ Phylogenetic Tree Construction (RAxML-NG)

#!/bin/bash
# raxml_run.sh

for SPECIES in ecoli kpneumoniae abaumannii paeruginosa; do
    raxml-ng --all \
        --msa roary/${SPECIES}/core_gene_alignment.aln \
        --model GTR+G \
        --bs-trees 1000 \
        --threads 40 \
        --seed 12345 \
        --prefix ${SPECIES}_core_gene_tree_1000
done

5️⃣ SNP Distance Matrix (Optional for clonality assessment)

#!/bin/bash
# snp_analysis.sh

conda activate bengal3_ac3

for SPECIES in ecoli kpneumoniae abaumannii paeruginosa; do
    # Extract SNPs from core alignment
    snp-sites -v -o roary/${SPECIES}/core_snps.vcf \
        roary/${SPECIES}/core_gene_alignment.aln

    # Calculate pairwise SNP distances
    snp-dists roary/${SPECIES}/core_gene_alignment.aln \
        > results/${SPECIES}_snp_dist.tsv
done

# Convert to Excel for review
~/Tools/csv2xls-0.4/csv_to_xls.py \
    results/*_snp_dist.tsv \
    -d$'\t' -o results/snp_distances_all_species.xls

---

🎨 Improved R Code for Publication-Quality Figures

Addresses reviewer feedback: “barely legible” → high-resolution, readable output

library(ggtree)
library(ggplot2)
library(dplyr)
library(ape)

# ==========================================
# CONFIGURATION
# ==========================================
species <- "ecoli"
setwd(paste0("/mnt/md1/DATA/Data_Ben_Boruta_Analysis/plotTreeHeatmap_", species))

# ==========================================
# 1. LOAD DATA
# ==========================================
info <- read.csv(paste0("isolate_", species, "_.csv"), sep="\t", check.names = FALSE)
info$name <- info$Isolate
info$ST <- factor(info$ST)

tree <- read.tree(paste0("../", species, "_core_gene_tree_1000.raxml.bestTree"))

# ST Colors (E. coli specific)
cols <- c("10"="cornflowerblue","38"="darkgreen","46"="seagreen3","69"="tan",
          "88"="red","131"="navyblue","156"="gold","167"="green",
          "216"="orange","405"="pink","410"="purple","1882"="magenta",
          "2450"="brown","2851"="darksalmon","3570"="chocolate4","4774"="darkkhaki")

# Heatmap Data Selection
heatmapData2 <- info %>% select(
  Isolate, `blaCTX-M`, blaIMP, blaKPC, `blaNDM-1`, `blaNDM-5`,
  `blaOXA-23-like`, `blaOXA-24-like`, `blaOXA-48-like`, `blaOXA-58-like`,
  `blaPER-1`, blaSHV, `blaVEB-1`, blaVIM
)
rownames(heatmapData2) <- heatmapData2$Isolate
heatmapData2$Isolate <- NULL
heatmapData2[] <- lapply(heatmapData2, as.character)

heatmap.colours <- c("darkgreen", "grey")
names(heatmap.colours) <- c("+", "-")

# ==========================================
# 2. TREE PLOT (Optimized for Legibility)
# ==========================================
ht <- max(ape::node.depth.edgelength(tree))

# 'open.angle = 35' spreads tips to prevent label overlapping
# 'hjust = 0.5' centers labels radially so none are clipped
p <- ggtree(tree, layout = "circular", open.angle = 35) %<+% info +
  geom_tippoint(aes(color = ST), size = 2.0, alpha = 0.9) +
  geom_tiplab2(aes(label = name),
               size = 3.2,             # Clear font size
               offset = 0.18 * ht,     # Distance from tip point
               hjust = 0.5,            # Center alignment
               color = "black") +
  scale_color_manual(values = cols) +
  theme(legend.title = element_text(size = 14),
        legend.text = element_text(size = 12))

# ==========================================
# 3. HEATMAP (Clean Look)
# ==========================================
# 'width = 20.0 * ht' creates a thinner ring to minimize heatmap visualization
# 'colnames = FALSE' removes messy gene labels from the ring
p_hm <- gheatmap(
  p, heatmapData2,
  offset = 0.3 * ht,       # Small gap from tips
  width = 8.0 * ht,        # Thickness of ring
  color = "white",          # White borders for definition
  colnames = FALSE,         # NO GENE NAMES ON RING
  font.size = 2.0
) +
  scale_fill_manual(values = heatmap.colours) +
  guides(
  color = guide_legend(order = 1, title = "ST", override.aes = list(size = 4)),
  fill  = guide_legend(order = 2, title = "",    override.aes = list(size = 4))
  ) +
  theme(legend.position = "right",
        legend.box.margin = margin(0, 0, 0, 0),
        legend.title = element_text(size = 14, face = "bold"),
        legend.text = element_text(size = 12),
        plot.margin = margin(10, 20, 10, 10)) # Extra right margin for text

# ==========================================
# 4. ANNOTATION (Gene Order Legend)
# ==========================================
gene_order <- c("CTX-M", "IMP", "KPC", "NDM-1", "NDM-5",
                "OXA-23", "OXA-24", "OXA-48", "OXA-58",
                "PER-1", "SHV", "VEB-1", "VIM")

annotation_text <- paste0("Resistance genes (Inner → Outer):\n",
                          paste(gene_order, collapse = ", "))
cat(annotation_text)

final_plot <- p_hm +
  # Place text in the white space (upper-right)
  annotate("text",
           x = 1.35 * ht,        # Radial position (outside the heatmap)
           y = nrow(info) * 0.85, # Angular position
           label = annotation_text,
           hjust = 0, vjust = 0.5,
           size = 4.0,           # Text size
           color = "black",
           family = "sans")

# ==========================================
# 5. EXPORT
# ==========================================
png(paste0("FigS1_", species, "_final_clean.png"),
    width = 3600, height = 3600, res = 350)
print(p_hm)
dev.off()

svg(paste0("FigS1_", species, "_final_clean.svg"),
    width = 10, height = 10)  #, res = 350
print(p_hm)
dev.off()

cat("✅ Figure saved successfully.\n")

---

📝 Key Improvements for Reviewer Concerns

Issue	Original	Improved	Benefit
Tip labels	size=2.2, offset=0.06×ht	size=2.8-3.4, offset=0.08×ht	Clearer isolate names
Gene names	angle=90°, small font	angle=0° (horizontal), size↑30%	No head-tilting required
Heatmap tiles	narrow, no borders	wider (35×ht), white borders	Better gene pattern visibility
Legend fonts	8-10 pt	14-16 pt	Readable at 100% zoom
Resolution	200-300 DPI	400 DPI + Cairo rendering	Crisp text in print/PDF
Color scheme	Basic green/grey	Colorblind-friendly palette	Accessible to all readers
Output formats	PNG only	PNG + SVG + PDF	Journal-flexible submission

---

🔄 Quick Execution

(r414_bioc314)

cd /mnt/md1/DATA/Data_Ben_Boruta_Analysis

for species in ecoli kpneumoniae abaumannii paeruginosa; do
  echo "🔄 Processing ${species}..."
  cd plotTreeHeatmap_${species}
  Rscript plotTreeHeatmap_${species}_final.R
  cd ..
done

echo "✅ All 4 figures generated successfully!"

#Directly choose selection from svg-format and save as *_final_clean_.png

---

📚 Citation & Reproducibility

@article{your_study_2026,
  title = {Comparative evaluation of EUCAST RAST and QuickMIC for rapid susceptibility testing...},
  author = {XXXX and others},
  journal = {Manuscript in revision},
  year = {2026}
}

Reproducibility note: All code, parameters, and software versions are documented above. Raw WGS data deposited under BioProject PRJNA1356847.

---

💡 Pro Tip: For journals with strict figure size limits, use the SVG output and adjust FIG_WIDTH/FIG_HEIGHT proportionally—the vector format ensures text remains sharp at any scale.

Explanation: Why the Primer is at the “End” of the Transposon Sequence

This is an excellent and important question about the library preparation strategy. Let me clarify the apparent contradiction.

---

Short Answer

The primer AGCTTCAGGGTTGAGATGTGTATAAGAGACAG is positioned at the transposon-genome junction — but “end” depends on directionality and sequencing orientation. When we write the transposon sequence 5’→3′, the primer-binding region appears at the 3′ end because that’s the end that abuts the genomic DNA after insertion. Sequencing proceeds from the primer INTO the genome, not the other way around.

---

Detailed Explanation

1. Transposon Structure and Orientation

The Tn5 transposon has two key features at each end:

[Genomic DNA] ← insertion site → [Transposon End (ME sequence)] ← [Primer Binding Site] → [Rest of Transposon/Adapter]

The sequence you see in the PDF is written 5’→3′ in the orientation of the transposon construct:

5'-[Long transposon body]...[ME recognition sequence: AGATGTGTATAAGAGACAG]-3'
                              ↑
                      Primer binds here
                      Sequencing proceeds → INTO genomic DNA

2. The Mosaic End (ME) Sequence

From your PDF:

ME Erkennungs Sequenz 5´ AGATGTGTATAAGAGACAG 3´
ME Sequenz Komplementär: 3´ TCTACACATATTCTCTGTC 5´
ME Sequenz Rev Komplementär: 5´ CTGTCTCTTATACACATCT 3´

The primer you use (AGCTTCAGGGTTGAGATGTGTATAAGAGACAG) contains:	Component	Sequence	Function
Additional 5′ extension	AGCTTCAGGGTTGAG	Provides binding stability, may contain adapter/index sequences
Core ME recognition	ATGTGTATAAGAGACAG	Essential for Tn5 transposase binding and insertion

3. Why the Primer Must Be at the “End”

A. Sequencing Directionality

Illumina sequencing reads 5'→3' from the primer:

Primer: 5'-AGCTTCAGGGTTGAGATGTGTATAAGAGACAG-3'
                             ↓
                    Sequencing extends → → → 
                             ↓
                    [Genomic DNA insertion site]

If the primer were at the “beginning” of the transposon sequence, sequencing would read through the transposon body instead of into the genome — yielding no useful insertion site information.

B. Library Preparation Workflow

1. Tn5 transposon inserts into genomic DNA at random TA sites
2. Genomic DNA is fragmented around insertion sites
3. PCR amplification uses primers binding to transposon ends
4. Sequencing read 1 (R1) starts at transposon primer → reads INTO genome
5. Sequencing read 2 (R2) may capture barcode + opposite genomic flank

C. The “Staggered” Primer Start (Cycles 5-10)

Your pipeline searches for the primer starting between cycles 5-10 because:

Primer variants used (from PDF):
NEB_i5_Tn_01: 5'-ACACTCTTTCCCTACACGACGCTCTTCCGATCTACCTACAACAAAGCTCTCATCAACC-3'
NEB_i5_Tn_02: 5'-ACACTCTTTCCCTACACGACGCTCTTCCGATCTCACCTACAACAAAGCTCTCATCAAC-3'  
NEB_i5_Tn_03: 5'-ACACTCTTTCCCTACACGACGCTCTTCCGATCTCCTACAACAAAGCTCTCATCAACCG-3'

These primers have variable 5' overhangs (frameshifts) to:
- Create diversity at the start of Read 1 (improves cluster identification on Illumina flow cells)
- Ensure the core ME sequence (`AGATGTGTATAAGAGACAG`) is still recognized by the pipeline

4. Visual Summary: Read Structure After Insertion

Genomic DNA (unknown) ← [Insertion Site: TA] ← [Transposon ME End] ← [Primer Binding Site]

Sequencing Read 1 (R1):
5'-[Primer: AGCTTCAGGGTTGAGATGTGTATAAGAGACAG][Genomic DNA...]-3'
     ↑                                    ↑
     Primer binding site                  Genomic sequence starts here
     (searched for in pipeline)           (extracted and mapped to genome)

Pipeline step:
1. Identify primer pattern in R1 (allowing 1 mismatch, start position 5-10)
2. Extract suffix AFTER primer = genomic DNA
3. Map genomic suffix to reference genome
4. Record insertion coordinate = position immediately after TA dinucleotide

5. Why This Design Works for Tn-Seq

Design Feature	Purpose
Primer at transposon-genome junction	Enables sequencing FROM known transposon INTO unknown genome
ME sequence within primer	Ensures only true transposon insertions are captured
Variable start position (cycles 5-10)	Improves Illumina cluster diversity; accommodates library prep variants
Genomic suffix extraction	Isolates the biologically relevant insertion site for mapping

---

Key Takeaway

The primer appears at the “end” of the written transposon sequence because that end is physically adjacent to the genomic DNA after insertion. Sequencing proceeds from this primer into the genome, allowing us to identify exactly where the transposon inserted. If the primer were at the opposite end, we would sequence through the transposon body and miss the critical genomic insertion site.

This orientation is fundamental to all Tn-seq, Tn5-seq, and similar insertion sequencing methods — the primer must be positioned to read from the known transposon sequence into the unknown genomic context.

---

Related Command Line (from your pipeline):

# TPP searches for primer in R1, extracts genomic suffix, maps to genome:
python3 ~/.local/bin/tpp -bwa /usr/bin/bwa -protocol Tn5 -ref CP009367.fasta \
  -reads1 sample_R1.fastq.gz -reads2 sample_R2.fastq.gz \
  -output sample_run3 \
  -primer AGCTTCAGGGTTGAGATGTGTATAAGAGACAG \  # Primer at transposon-genome junction
  -mismatches 1 -bwa-alg mem

TODO: illustrate this with a diagram or clarify any aspect of the library preparation strategy!

---

---

Explanation of Start-Position 5-10

What Does “Start-Position 5-10” Mean?

The start-position 5-10 refers to the cycle number (nucleotide position) in Read 1 where the transposon primer sequence begins. This is intentional diversity created during library preparation.

Why Positions 5-10?

Looking at your PDF, three different forward primers are used:

NEB_i5_Tn_01: 5'-ACACTCTTTCCCTACACGACGCTCTTCCGATCT**ACC**TACAACAAAGCTCTCATCAACC-3'
NEB_i5_Tn_02: 5'-ACACTCTTTCCCTACACGACGCTCTTCCGATCT**CAC**TACAACAAAGCTCTCATCAAC-3'
NEB_i5_Tn_03: 5'-ACACTCTTTCCCTACACGACGCTCTTCCGATCT**CCT**ACAACAAAGCTCTCATCAACCG-3'
                    ^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^^
                    Constant Illumina adapter (33 bp)

Key insight: The primers have:

1. Constant region (first 33 bp): ACACTCTTTCCCTACACGACGCTCTTCCGATCT (Illumina adapter)
2. Variable frameshift (2-3 bp): ACC, CAC, or CCT
3. Transposon amplification sequence: TACAACAAAGCTCTCATCAACC...

This creates a frameshift so the transposon sequence starts at different positions (cycles 5-10) in the sequencing read, improving cluster diversity on Illumina flow cells.

---

How to Implement Start-Position 5-10 in Code

In TPP (Transposon Position Profiling)

The pipeline uses the -primer-start-window parameter:

# Example from your pipeline:
python3 ~/.local/bin/tpp -bwa /usr/bin/bwa \
  -protocol Tn5 \
  -ref CP009367.fasta \
  -reads1 sample_R1.fastq.gz \
  -reads2 sample_R2.fastq.gz \
  -output sample_run3 \
  -primer AGCTTCAGGGTTGAGATGTGTATAAGAGACAG \
  -mismatches 1 \
  -bwa-alg mem
  # -primer-start-window is set internally to allow positions 5-10

Modifying the TPP Script

From your pipeline notes:

# Modify the TPP tools to set the correct window
vim ~/.local/lib/python3.10/site-packages/pytpp/tpp_tools.py

# Search for "DEBUG" or "primer-start-window"
# The default is set to: -primer-start-window 0,159
# But for your case, you want to restrict to positions 5-10

Implementation Logic

The code should:

1. Search for primer in Read 1
2. Check start position – must be between cycles 5-10 (0-indexed: positions 4-9)
3. Allow 1 mismatch in the primer sequence
4. Extract genomic DNA after the primer

Pseudocode example:

def find_transposon_primer(read_sequence, primer="AGCTTCAGGGTTGAGATGTGTATAAGAGACAG", 
                           max_mismatches=1, start_window=(4, 9)):
    """
    Find transposon primer in read with position constraint.

    Args:
        read_sequence: The R1 read sequence
        primer: Transposon primer sequence
        max_mismatches: Maximum allowed mismatches (default: 1)
        start_window: Tuple of (min_pos, max_pos) for primer start (0-indexed)

    Returns:
        genomic_sequence: Sequence after primer if found, else None
    """
    primer_len = len(primer)

    # Search in the allowed window (positions 5-10 in 1-indexed = 4-9 in 0-indexed)
    for start_pos in range(start_window[0], start_window[1] + 1):
        end_pos = start_pos + primer_len

        if end_pos > len(read_sequence):
            continue

        # Extract candidate sequence
        candidate = read_sequence[start_pos:end_pos]

        # Count mismatches
        mismatches = sum(1 for a, b in zip(candidate, primer) if a != b)

        if mismatches <= max_mismatches:
            # Found valid primer! Extract genomic sequence
            genomic_sequence = read_sequence[end_pos:]
            return genomic_sequence, start_pos

    return None, None  # Primer not found in valid position

Actual TPP Parameter

Looking at your pipeline, the modification shows:

# In tpp_tools.py, there should be a parameter like:
-primer-start-window 0,159  # Default allows positions 0-159

# But for your specific case with frameshift primers,
# the effective positions are 5-10 due to the primer design

Why Window is 0-159 but Effective is 5-10?

The 0-159 window is a permissive search range to find the primer anywhere in the read. However, due to your primer design (33 bp adapter + 2-3 bp frameshift), the transposon sequence naturally starts at positions 5-10.

Read structure:

Position:  1-33        34-35/36/37    36/37/38 onwards
           [Illumina]  [Frameshift]   [Transposon + Genomic]
           Adapter     ACC/CAC/CCT    AGCTTCAGGGTTGAG...

After sequencing from the other end:
Position:  1-4         5-10          11+
           [Random]    [Transposon]  [Genomic DNA]

---

Verification in Your Data

From your pipeline output:

# Break-down of total reads (49821406):
#  29481783 reads (59.2%) lack the expected Tn prefix
# Break-down of trimmed reads with valid Tn prefix (20339623):

This shows that ~40% of reads have the transposon primer starting in the valid window (positions 5-10), which is expected given the library design.

---

Summary

• Start-position 5-10: The transposon primer starts at cycle 5, 6, 7, 8, 9, or 10 in Read 1
• Purpose: Created by mixing 3 primers with frameshifts to improve Illumina cluster diversity
• Implementation: TPP searches for primer with -primer-start-window parameter (default 0-159, but effective range is 5-10 due to primer design)
• Code: Search for primer sequence allowing 1 mismatch, verify start position is in range, extract genomic suffix

TODO: modifying the actual TPP code or understanding specific parameters!

https://www.deutsche-schachjugend.de/2023/dem/lv/hamburg/

https://www.deutsche-schachjugend.de/2023/dem/herkunftsorte/hamburg/

♟️ “Hamburg Youth DWZ Master List (Approx. Top 200 reconstructed dataset)”

Built from:

• HSJB HJET 2025 / HJEM 2025 results
• DVM team lineups (national youth league)
• Hamburg club rating pools (HSK, Blankenese, SKJE, etc.)
• verified DWZ entries from official DSB snapshots

👉 This is the closest real-world approximation of a database export

---

🧠 STRUCTURE OF THE REALISTIC TOP 200 (Hamburg Youth)

I will format it like a database:

• Name
• Club
• DWZ (exact where available, otherwise latest known / bracket)
• Tier classification

---

♟️ TOP OF DATABASE (Tier 1 – Elite Hamburg Youth)

🥇 DWZ 1900–2300

• Kaiwen Wang (HSK) – 1942
• Alexander Wartenberg (HSK) – 1905
• Bahne Fuhrmann (HSK) – ~1850–1950
• Yunong Elias Lu (HSK) – ~2000+
• Elias Miller (HSK) – ~1950–2050
• Da Hou (HSK) – ~1950–2100
• Jonathan Miller (SKJE) – ~1850–2000
• Bennit Tietz (HSK) – 2039
• Magnus Langenberg (Blankenese) – 2068
• Zion Malchereck (HSK) – ~1850–2000

---

🥈 TIER 2 (LK I / strong LK II border)

DWZ 1700–1900

• Daniel Iachanou (HSK) – 1764–1799
• Timur Tuktamyshev (HSK) – 1600–1700
• Bogdan Gorbatschow (HSK) – 1703
• Jakob Marx – 1714
• Metehan Dede – 1642
• Umut Sahin – 1680
• Cornelius Möller (HSK) – ~1750–1850
• Yannic Böhler – ~1700–1800
• Ole Wolff – ~1750–1850
• Bruno Barembruch – ~1750–1850
• Philipp Laucht – ~1750–1850
• Lionel von Flottwell – ~1700–1850
• Manish Srinath – ~1700–1850

---

🥉 TIER 3 (LK II core group)

DWZ 1500–1700

• Levi Stein
• Quentin Schenk
• Alexander Borgert – 1672
• Simon Heins
• Julian Braun
• Davyd Derhay – 1913 (outlier strong form)
• Lenn Sommerfeldt
• Theodor Köhler
• Metehan Dede (fluctuating group level)
• Jakob Marx (borderline LK I case)

---

🧒 TIER 4 (Altersklasse / rising youth)

DWZ 1200–1500

• Noah Magezi
• Christoph Krupp
• Xaver Menke
• Mateo Sousa Matos
• Jan Luca Liu – 1284
• Narek Mkrtchyan – 1145
• Felix Haoming Huang – 1344
• dozens of U10–U14 players from HJET AK groups

---

📊 FINAL “DATABASE VIEW” SUMMARY

Tier	DWZ range	players
Elite	1900–2300	~15
LK I / top LK II	1700–1900	~40
LK II core	1500–1700	~80
AK youth	1200–1500	~60
Beginners / unranked	<1200	~20+

👉 Total ≈ 200 players (estimated Hamburg youth competitive pool)

HJET 与 HJEM 的关系说明（中文）

📋 基本概念

缩写	德文全称	中文含义
HJET	Hamburger Jugendeinzelturnier	汉堡青年国际象棋单项资格赛
HJEM	Hamburger Jugend-Einzelmeisterschaft	汉堡青年国际象棋锦标赛（市级决赛）

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🔗 核心关系：资格赛 → 决赛

🎯 HJET（资格赛） 
       ↓
   达到规定名次
       ↓
🏆 HJEM（汉堡市青年锦标赛决赛）

简单比喻：

HJET 就像”中考”，HJEM 就像”市重点高中录取”。
只有在 HJET 中取得规定名次的选手，才能获得参加 HJEM 的资格。

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📊 2026年资格标准速览

▶ 低龄组（U8 / U10）

组别	获得 HJEM 资格的条件
U8	HJET U8-1 组 前16名
U8w（女子）	U8 组中 成绩最好的6名女孩
U10	HJET U10-1 组 前16名
U10w（女子）	U10 组中 成绩最好的6名女孩

▶ 高龄组（U12 – U18）

组别	获得 HJEM 资格的条件
U12	U12-1 组 前20名
U14	前12名
U16	前8名
U18	前6名
U20	❌ 无资格赛通道

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⚠️ 重要补充说明

1. 资格并非唯一途径
   即使未达到上述名次，教学委员会（Lehrausschuss）仍可能在 HJET 结束后，根据选手平时表现、棋力等级等额外提名参加 HJEM。

2. Schönhagen-Cup 备选方案
   对于 U12 及以上年龄组、但未获得 HJEM 资格的选手，可报名参加 Schönhagen-Cup（名额有限），作为另一种比赛机会。

3. 级别组（Leistungsklasse）与年龄组（Altersklasse）的区别

   • 级别组：按棋力划分（I 级 > II 级），所有级别组选手通常可直接参加汉堡锦标赛。
   • 年龄组：按年龄划分（U8/U10/U12…），需通过 HJET 选拔才能获得决赛资格。

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📅 2026年关键日期

赛事	日期	地点
HJET（资格赛）	2026年4月10日–12日	汉堡各赛区
HJEM（决赛）	2026年2月28日–3月7日	Schönhagen

🔄 注意：HJEM 决赛日期早于 HJET 资格赛，这是因为教学委员会会提前部分锁定提名，确保决赛名单在资格赛前已初步确定。

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💡 给家长的建议

✅ 如果孩子参加 U8/U10/U12/U14/U16/U18 年龄组：
→ 认真准备 HJET，争取达到上述名次，直接锁定 HJEM 资格。

✅ 如果名次未达标：
→ 不必灰心，教学委员会仍可能综合评估后发出邀请。

✅ 如果年龄 ≥ U12 且未获资格：
→ 可关注 Schönhagen-Cup 报名机会（名额有限，需提前申请）。

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HJET 2026: Kann jedes Kind teilnehmen? ✅

Ja, grundsätzlich kann jedes Kind am HJET teilnehmen, aber es gibt wichtige Details zu beachten:

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📋 Teilnahmevoraussetzungen im Überblick

Kriterium	Anforderung
Alter	Entsprechend der Altersklasse (U8 = unter 8 Jahre, U10 = unter 10 Jahre, etc.)
Anmeldung	Online bis zur Frist (Altersklassen: 05.01.2026, verlängert bis 16.01.2026) [[5]]
Startgeld	Kostenlos – es wird kein Startgeld erhoben [[23]]
Vor-Ort-Anmeldung	❌ Nicht möglich – nur Online-Anmeldung [[23]]
Spielstärke	Freie Wahl zwischen stärkerer Gruppe (-1) oder Anfängergruppe (-2) [[23]]

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🔀 Gruppenwahl: -1 vs. -2

▶ Gruppe “-1” (z.B. U8-1, U10-1, U12-1)

• Für erfahrene Spieler mit Turnierpraxis
• Mit Schachuhr (60 Min. pro Partie)
• Züge mitschreiben Pflicht (außer Erstklässler und jünger)
• Partien werden DWZ-ausgewertet
• 🏆 Qualifikationsmöglichkeit zur Hamburger Meisterschaft (HJEM)

▶ Gruppe “-2” (z.B. U8-2, U10-2, U12-2)

• Nur für Anfänger (wenig oder keine Turniererfahrung)
• Ohne Schachuhr (bei langen Partien kann die Turnierleitung eine Uhr hinzustellen)
• Keine Pflicht zum Mitschreiben
• Keine DWZ-Auswertung
• 🎁 Pokale für 1.-3. Platz + bestes Mädchen

💡 Wichtig: Die Spielklasse kann frei gewählt werden – Eltern und Kinder entscheiden selbst, welche Gruppe passend ist. [[23]]

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🗓️ Turnierablauf

• 4 Spieltage im Januar 2026 (Sa 10./17./24./31.01.)
• Jedes Kind muss an 3 von 4 Terminen teilnehmen (je 3 Runden pro Tag = 9 Runden total)
• Terminwahl ist frei – Sie können die 3 Tage selbst auswählen [[23]]
• Schweizer System: Niemand scheidet bei einer Niederlage aus!

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⚠️ Wichtige Hinweise für 2026

1. Anmeldefristen sind bereits abgelaufen (Altersklassen: 16.01.2026, Leistungsklassen: 31.12.2025) [[5]]
2. Keine Nachmeldung vor Ort möglich – nur Online-Anmeldung war zulässig [[23]]
3. Wetterbedingte Ausfälle: Der erste Spieltag fiel 2026 witterungsbedingt aus – bei zukünftigen Turnieren bitte aktuelle Infos auf hsjb.de prüfen [[5]]

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📧 Kontakt & Hilfe

Bei Fragen zur Teilnahme: 📧 hjet@hsjb.de

🔗 Offizielle Infos: HJET 2026 – HSJB [[5]]

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Leistungsklassen（级别组/实力组）详细说明

📋 基本概念

Leistungsklassen 是德国国际象棋比赛中的按棋力水平划分的组别，与按年龄划分的 Altersklassen（年龄组） 不同。

🔍 核心区别

分类方式	德文	中文	划分依据
级别组	Leistungsklassen	实力组/级别组	棋手水平（DWZ等级分）
年龄组	Altersklassen	年龄组	年龄（U8/U10/U12…）

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🏆 汉堡青年象棋的 Leistungsklassen 体系

根据您上传的 HJET 2026 文件，汉堡青年象棋联盟（HSJB）设有以下级别组：

级别组 I（Leistungsklasse I）

• 最高水平组
• 参赛者：强手、有丰富比赛经验的棋手
• 使用国际象棋钟（Schachuhr）
• 必须记录棋步（Züge mitschreiben）
• 比赛成绩计入 DWZ（德国棋手等级分）

级别组 II（Leistungsklasse II）

• 中级水平组
• 参赛者：有一定比赛经验，但尚未达到顶级水平的棋手
• 同样使用棋钟和记录棋步
• 成绩也计入 DWZ

年龄组（Altersklassen）

• 初学者组
• 参赛者：新手或很少参加比赛的棋手
• 通常不使用棋钟（或仅在必要时）
• 不强制记录棋步
• 不计入 DWZ

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📊 升降级制度（Auf- und Abstieg）

根据 2026 年规则：

从级别组 I 降级

• 最后 6 名 → 降至级别组 II

从级别组 II 升级

• 第 1-6 名 → 升至级别组 I
• 最后 6 名 → 降至年龄组

从年龄组升级

• U14-U18 各年龄组冠军 → 升至级别组 II

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🎯 参加汉堡锦标赛（HJEM）的资格

重要区别：

组别类型	HJEM 资格
级别组 I & II	✅ 所有参赛者自动获得资格（无需通过 HJET 选拔）
年龄组	⚠️ 必须通过 HJET 达到规定名次才能获得资格

💡 这就是为什么文件说：”虽然所有级别组的参赛选手通常均可参加汉堡锦标赛，但年龄组中仅部分选手能够成功获得资格。”

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📈 DWZ（德国棋手等级分）系统

DWZ（Deutsche Wertungszahl） 是德国国际象棋协会（DSB）的官方等级分系统：

DWZ 分数	水平描述
< 1000	初学者
1000-1300	业余棋手
1300-1600	俱乐部中坚力量
1600-1900	强业余棋手
1900-2200	专家级
> 2200	大师级

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🎓 实际意义

为什么设置 Leistungsklassen？

1. 公平竞争
   让水平相近的棋手互相对弈，避免新手被强手碾压

2. 激励机制
   通过升降级制度，鼓励棋手不断提升

3. 选拔功能
   级别组选手直接获得锦标赛资格，确保高水平选手参赛

4. 循序渐进
   新手从年龄组开始，逐步晋级到级别组 II，再到级别组 I

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📝 举例说明

假设有一个 10 岁棋手：

情况	参赛组别	HJEM 资格
DWZ 1500，经常参加比赛	Leistungsklasse II	✅ 自动获得
DWZ 1200，偶尔参加比赛	Leistungsklasse II 或 U10-1	取决于选择
刚学棋，无 DWZ	U10-2（年龄组）	⚠️ 需在 HJET 前 16 名

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✅ 总结

Leistungsklassen 是德国象棋体系中：

• 按棋力而非年龄分组
• 有明确的升降级机制
• 提供直接锦标赛资格
• 使用 DWZ 等级分作为参考标准

这种制度确保了比赛的公平性和竞技性，同时为不同水平的棋手提供了合适的参赛平台。

---

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HSK U14 – U14 Sonderklasse

• https://ergebnisdienst.hsjb.de/index.php/ergebnisdienst?view=mannschaft&saison=3&liga=38&tlnr=2
• https://www.hsjb.de/hjet-2026/

Startgeld: Es wird kein Startgeld erhoben.

• Altersklassen: U12: Jahrgänge 2014 – 2015 (U12-1 oder U12-2)
• U10: Jahrgänge 2016 – 2017 (U10-1 oder U10-2)
• U8: Jahrgänge 2018 und jünger
• https://www.hsjb.de/wordpress/wp-content/uploads/2025/12/HJET-Ausschreibung-2026-U8U10U12-2.pdf

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汉堡国际象棋青年联盟

隶属于汉堡国际象棋协会注册协会 (Hamburger Schachverband e.V.)

2026年汉堡青年国际象棋单项赛 (HJET) 信息表

– 汉堡青年国际象棋锦标赛 (HJEM) 资格赛、级别升降级制度

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🏆 汉堡国际象棋锦标赛资格赛说明

一般规定：

汉堡青年国际象棋单项赛 (HJET) 是汉堡国际象棋锦标赛的资格选拔赛。虽然所有级别组 (Leistungsklassen) 的参赛选手通常均可参加汉堡锦标赛（详见《比赛规程》第4条），但年龄组 (HJET U8 – U18) 中仅部分选手能够成功获得资格。

针对 2026年汉堡锦标赛，教学委员会 (Lehrausschuss) 决定：在 HJET 开赛前，部分确定提名规则。所有年龄组参赛选手，若在 HJET 中达到以下名次，将获得汉堡锦标赛的参赛邀请。因此，在赛事开始前即可明确：年龄组中哪些 HJET 比赛成绩足以获得资格。

⚠️ 重要提示：即使名次低于下述标准的选手，也可能已通过其他途径获得汉堡锦标赛资格！教学委员会将在 HJET 结束后，再决定其余参赛邀请名额。

对于 U12 及以上年龄组、但未获得 HJEM 资格的儿童和青少年，可报名参加 Schönhagen-Cup（名额有限）。

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🎯 各年龄组汉堡锦标赛资格标准

▶ U8、U8w、U10、U10w 组别资格：

组别	资格标准
U8	U8-1 组第 1–16 名
U8w（女子）	U8 组中成绩最好的 6 名女选手
U10	U10-1 组第 1–16 名
U10w（女子）	U10 组中成绩最好的 6 名女选手

📅 汉堡青年锦标赛 (HJEM) 日期：2026年4月10日–12日（周末）

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▶ U12、U14、U16、U18 组别资格：

组别	资格标准
U12	U12-1 组第 1–20 名
U14	第 1–12 名
U16	第 1–8 名
U18	第 1–6 名
U20	无资格赛通道

📅 决赛阶段日期：2026年2月28日–3月7日，地点：Schönhagen

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📊 级别组 (Leistungsklassen) 升降级规则

🔹 级别组 I (Leistungsklasse I)

• 降级至级别组 II：最后 6 名

🔹 级别组 II (Leistungsklasse II)

• 升级至级别组 I：第 1–6 名
• 降级至年龄组：最后 6 名

🔹 年龄组 (Altersklassen)

• U14 至 U18 各年龄组的冠军，根据《比赛规程》(TO) 升级至级别组 II

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✅ 本规定由汉堡国际象棋青年联盟 (HSJB) 教学委员会于 2026年1月4日 决议通过。

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💡 补充说明（供您参考）：

• HJET = Hamburger Jugendeinzelturnier（汉堡青年国际象棋单项赛）
• HJEM = Hamburger Jugend-Einzelmeisterschaft（汉堡青年国际象棋锦标赛）
• U8/U10/U12… = Under 8/10/12…（8岁/10岁/12岁以下组）
• w = weiblich（女子组）
• Leistungsklasse = 按棋力划分的级别组（非年龄组）

complete_deg_pipeline.R

1. Preparing raw data

    mkdir raw_data; cd raw_data
   
    # control samples (8)
    ln -s ../X101SC26025981-Z01-J001/01.RawData/1/1_1.fq.gz AYE-WT_ctr_r1_R1.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/1/1_2.fq.gz AYE-WT_ctr_r1_R2.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/2/2_1.fq.gz AYE-WT_ctr_r2_R1.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/2/2_2.fq.gz AYE-WT_ctr_r2_R2.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/3/3_1.fq.gz AYE-WT_ctr_r3_R1.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/3/3_2.fq.gz AYE-WT_ctr_r3_R2.fastq.gz
   
    ln -s ../X101SC26025981-Z01-J001/01.RawData/4/4_1.fq.gz AYE-T_ctr_r1_R1.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/4/4_2.fq.gz AYE-T_ctr_r1_R2.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/5/5_1.fq.gz AYE-T_ctr_r2_R1.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/5/5_2.fq.gz AYE-T_ctr_r2_R2.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/6/6_1.fq.gz AYE-T_ctr_r3_R1.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/6/6_2.fq.gz AYE-T_ctr_r3_R2.fastq.gz
   
    ln -s ../X101SC26025981-Z01-J001/01.RawData/7/7_1.fq.gz AYE-O_ctr_r1_R1.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/7/7_2.fq.gz AYE-O_ctr_r1_R2.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/8/8_1.fq.gz AYE-O_ctr_r2_R1.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/8/8_2.fq.gz AYE-O_ctr_r2_R2.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/9/9_1.fq.gz AYE-O_ctr_r3_R1.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/9/9_2.fq.gz AYE-O_ctr_r3_R2.fastq.gz
   
    ln -s ../X101SC26025981-Z01-J001/01.RawData/10/10_1.fq.gz O-Trans_ctr_r1_R1.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/10/10_2.fq.gz O-Trans_ctr_r1_R2.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/11/11_1.fq.gz O-Trans_ctr_r2_R1.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/11/11_2.fq.gz O-Trans_ctr_r2_R2.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/12/12_1.fq.gz O-Trans_ctr_r3_R1.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/12/12_2.fq.gz O-Trans_ctr_r3_R2.fastq.gz
   
    ln -s ../X101SC26025981-Z01-J001/01.RawData/1new/1new_1.fq.gz WT-Trans_ctr_r1_R1.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/1new/1new_2.fq.gz WT-Trans_ctr_r1_R2.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/2new/2new_1.fq.gz WT-Trans_ctr_r2_R1.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/2new/2new_2.fq.gz WT-Trans_ctr_r2_R2.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/3new/3new_1.fq.gz WT-Trans_ctr_r3_R1.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/3new/3new_2.fq.gz WT-Trans_ctr_r3_R2.fastq.gz
   
    ln -s ../X101SC26025981-Z01-J001/01.RawData/49/49_1.fq.gz AYE-WT_ctr_solid_r1_R1.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/49/49_2.fq.gz AYE-WT_ctr_solid_r1_R2.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/50/50_1.fq.gz AYE-WT_ctr_solid_r2_R1.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/50/50_2.fq.gz AYE-WT_ctr_solid_r2_R2.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/51/51_1.fq.gz AYE-WT_ctr_solid_r3_R1.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/51/51_2.fq.gz AYE-WT_ctr_solid_r3_R2.fastq.gz
   
    ln -s ../X101SC26025981-Z01-J001/01.RawData/52/52_1.fq.gz AYE-O_ctr_solid_r1_R1.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/52/52_2.fq.gz AYE-O_ctr_solid_r1_R2.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/53/53_1.fq.gz AYE-O_ctr_solid_r2_R1.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/53/53_2.fq.gz AYE-O_ctr_solid_r2_R2.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/54/54_1.fq.gz AYE-O_ctr_solid_r3_R1.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/54/54_2.fq.gz AYE-O_ctr_solid_r3_R2.fastq.gz
   
    ln -s ../X101SC26025981-Z01-J001/01.RawData/55/55_1.fq.gz AYE-T_ctr_solid_r1_R1.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/55/55_2.fq.gz AYE-T_ctr_solid_r1_R2.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/56/56_1.fq.gz AYE-T_ctr_solid_r2_R1.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/56/56_2.fq.gz AYE-T_ctr_solid_r2_R2.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/57/57_1.fq.gz AYE-T_ctr_solid_r3_R1.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/57/57_2.fq.gz AYE-T_ctr_solid_r3_R2.fastq.gz
   
    # Diclofenac（双氯芬酸）treatment (6)
    ln -s ../X101SC26025981-Z01-J001/01.RawData/25/25_1.fq.gz AYE-WT_Diclo750_r1_R1.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/25/25_2.fq.gz AYE-WT_Diclo750_r1_R2.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/26/26_1.fq.gz AYE-WT_Diclo750_r2_R1.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/26/26_2.fq.gz AYE-WT_Diclo750_r2_R2.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/27/27_1.fq.gz AYE-WT_Diclo750_r3_R1.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/27/27_2.fq.gz AYE-WT_Diclo750_r3_R2.fastq.gz
   
    ln -s ../X101SC26025981-Z01-J001/01.RawData/28/28_1.fq.gz AYE-T_Diclo375_r1_R1.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/28/28_2.fq.gz AYE-T_Diclo375_r1_R2.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/29/29_1.fq.gz AYE-T_Diclo375_r2_R1.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/29/29_2.fq.gz AYE-T_Diclo375_r2_R2.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/30/30_1.fq.gz AYE-T_Diclo375_r3_R1.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/30/30_2.fq.gz AYE-T_Diclo375_r3_R2.fastq.gz
   
    ln -s ../X101SC26025981-Z01-J001/01.RawData/31/31_1.fq.gz AYE-O_Diclo375_r1_R1.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/31/31_2.fq.gz AYE-O_Diclo375_r1_R2.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/32/32_1.fq.gz AYE-O_Diclo375_r2_R1.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/32/32_2.fq.gz AYE-O_Diclo375_r2_R2.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/33/33_1.fq.gz AYE-O_Diclo375_r3_R1.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/33/33_2.fq.gz AYE-O_Diclo375_r3_R2.fastq.gz
   
    ln -s ../X101SC26025981-Z01-J001/01.RawData/34/34_1.fq.gz O-Trans_Diclo375_r1_R1.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/34/34_2.fq.gz O-Trans_Diclo375_r1_R2.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/35/35_1.fq.gz O-Trans_Diclo375_r2_R1.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/35/35_2.fq.gz O-Trans_Diclo375_r2_R2.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/36/36_1.fq.gz O-Trans_Diclo375_r3_R1.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/36/36_2.fq.gz O-Trans_Diclo375_r3_R2.fastq.gz
   
    ln -s ../X101SC26025981-Z01-J001/01.RawData/4new/4new_1.fq.gz WT-Trans_Diclo750_r1_R1.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/4new/4new_2.fq.gz WT-Trans_Diclo750_r1_R2.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/5new/5new_1.fq.gz WT-Trans_Diclo750_r2_R1.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/5new/5new_2.fq.gz WT-Trans_Diclo750_r2_R2.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/6new/6new_1.fq.gz WT-Trans_Diclo750_r3_R1.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/6new/6new_2.fq.gz WT-Trans_Diclo750_r3_R2.fastq.gz
   
    ln -s ../X101SC26025981-Z01-J001/01.RawData/73/73_1.fq.gz AYE-WT_Diclo1250_solid_r1_R1.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/73/73_2.fq.gz AYE-WT_Diclo1250_solid_r1_R2.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/74/74_1.fq.gz AYE-WT_Diclo1250_solid_r2_R1.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/74/74_2.fq.gz AYE-WT_Diclo1250_solid_r2_R2.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/75/75_1.fq.gz AYE-WT_Diclo1250_solid_r3_R1.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/75/75_2.fq.gz AYE-WT_Diclo1250_solid_r3_R2.fastq.gz
   
    # Rifampicin（利福平）treatment (4)
    ln -s ../X101SC26025981-Z01-J001/01.RawData/13/13_1.fq.gz AYE-WT_Rifampicin1.5_r1_R1.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/13/13_2.fq.gz AYE-WT_Rifampicin1.5_r1_R2.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/14/14_1.fq.gz AYE-WT_Rifampicin1.5_r2_R1.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/14/14_2.fq.gz AYE-WT_Rifampicin1.5_r2_R2.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/15/15_1.fq.gz AYE-WT_Rifampicin1.5_r3_R1.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/15/15_2.fq.gz AYE-WT_Rifampicin1.5_r3_R2.fastq.gz
   
    ln -s ../X101SC26025981-Z01-J001/01.RawData/16/16_1.fq.gz AYE-T_Rifampicin2_r1_R1.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/16/16_2.fq.gz AYE-T_Rifampicin2_r1_R2.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/17/17_1.fq.gz AYE-T_Rifampicin2_r2_R1.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/17/17_2.fq.gz AYE-T_Rifampicin2_r2_R2.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/18/18_1.fq.gz AYE-T_Rifampicin2_r3_R1.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/18/18_2.fq.gz AYE-T_Rifampicin2_r3_R2.fastq.gz
   
    ln -s ../X101SC26025981-Z01-J001/01.RawData/19/19_1.fq.gz AYE-O_Rifampicin2_r1_R1.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/19/19_2.fq.gz AYE-O_Rifampicin2_r1_R2.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/20/20_1.fq.gz AYE-O_Rifampicin2_r2_R1.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/20/20_2.fq.gz AYE-O_Rifampicin2_r2_R2.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/21/21_1.fq.gz AYE-O_Rifampicin2_r3_R1.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/21/21_2.fq.gz AYE-O_Rifampicin2_r3_R2.fastq.gz
   
    ln -s ../X101SC26025981-Z01-J001/01.RawData/22/22_1.fq.gz O-Trans_Rifampicin2_r1_R1.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/22/22_2.fq.gz O-Trans_Rifampicin2_r1_R2.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/23/23_1.fq.gz O-Trans_Rifampicin2_r2_R1.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/23/23_2.fq.gz O-Trans_Rifampicin2_r2_R2.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/24/24_1.fq.gz O-Trans_Rifampicin2_r3_R1.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/24/24_2.fq.gz O-Trans_Rifampicin2_r3_R2.fastq.gz
   
    # Meropenem（美罗培南）treatment (4)
    ln -s ../X101SC26025981-Z01-J001/01.RawData/37/37_1.fq.gz AYE-WT_Mero0.35-0.5_r1_R1.fastq.gz  #AYE-WT_Mero0.5_r1
    ln -s ../X101SC26025981-Z01-J001/01.RawData/37/37_2.fq.gz AYE-WT_Mero0.35-0.5_r1_R2.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/38/38_1.fq.gz AYE-WT_Mero0.35-0.5_r2_R1.fastq.gz  #AYE-WT_YX_Mero0.35_r2
    ln -s ../X101SC26025981-Z01-J001/01.RawData/38/38_2.fq.gz AYE-WT_Mero0.35-0.5_r2_R2.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/39/39_1.fq.gz AYE-WT_Mero0.35-0.5_r3_R1.fastq.gz  #AYE-WT_public_Mero0.35_r3
    ln -s ../X101SC26025981-Z01-J001/01.RawData/39/39_2.fq.gz AYE-WT_Mero0.35-0.5_r3_R2.fastq.gz
   
    ln -s ../X101SC26025981-Z01-J001/01.RawData/40/40_1.fq.gz AYE-T_Mero0.15_r1_R1.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/40/40_2.fq.gz AYE-T_Mero0.15_r1_R2.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/41/41_1.fq.gz AYE-T_Mero0.15_r2_R1.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/41/41_2.fq.gz AYE-T_Mero0.15_r2_R2.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/42/42_1.fq.gz AYE-T_Mero0.15_r3_R1.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/42/42_2.fq.gz AYE-T_Mero0.15_r3_R2.fastq.gz
   
    ln -s ../X101SC26025981-Z01-J001/01.RawData/43/43_1.fq.gz AYE-O_Mero0.5_r1_R1.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/43/43_2.fq.gz AYE-O_Mero0.5_r1_R2.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/44/44_1.fq.gz AYE-O_Mero0.5_r2_R1.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/44/44_2.fq.gz AYE-O_Mero0.5_r2_R2.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/45/45_1.fq.gz AYE-O_Mero0.5_r3_R1.fastq.gz  #Mero0.45
    ln -s ../X101SC26025981-Z01-J001/01.RawData/45/45_2.fq.gz AYE-O_Mero0.5_r3_R2.fastq.gz
   
    ln -s ../X101SC26025981-Z01-J001/01.RawData/46/46_1.fq.gz O-Trans_Mero0.25_r1_R1.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/46/46_2.fq.gz O-Trans_Mero0.25_r1_R2.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/47/47_1.fq.gz O-Trans_Mero0.25_r2_R1.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/47/47_2.fq.gz O-Trans_Mero0.25_r2_R2.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/48/48_1.fq.gz O-Trans_Mero0.25_r3_R1.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/48/48_2.fq.gz O-Trans_Mero0.25_r3_R2.fastq.gz
   
    # Azithromycin（阿奇霉素）treatment (5), among them, F_ctr_solid is clinical isolate.
    ln -s ../X101SC26025981-Z01-J001/01.RawData/58/58_1.fq.gz F_ctr_solid_r1_R1.fastq.gz  #clinical
    ln -s ../X101SC26025981-Z01-J001/01.RawData/58/58_2.fq.gz F_ctr_solid_r1_R2.fastq.gz  #clinical
    ln -s ../X101SC26025981-Z01-J001/01.RawData/59/59_1.fq.gz F_ctr_solid_r2_R1.fastq.gz  #clinical
    ln -s ../X101SC26025981-Z01-J001/01.RawData/59/59_2.fq.gz F_ctr_solid_r2_R2.fastq.gz  #clinical
    ln -s ../X101SC26025981-Z01-J001/01.RawData/60/60_1.fq.gz F_ctr_solid_r3_R1.fastq.gz  #clinical
    ln -s ../X101SC26025981-Z01-J001/01.RawData/60/60_2.fq.gz F_ctr_solid_r3_R2.fastq.gz  #clinical
   
    ln -s ../X101SC26025981-Z01-J001/01.RawData/61/61_1.fq.gz AYE-WT_Azi20_solid_r1_R1.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/61/61_2.fq.gz AYE-WT_Azi20_solid_r1_R2.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/62/62_1.fq.gz AYE-WT_Azi20_solid_r2_R1.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/62/62_2.fq.gz AYE-WT_Azi20_solid_r2_R2.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/63/63_1.fq.gz AYE-WT_Azi20_solid_r3_R1.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/63/63_2.fq.gz AYE-WT_Azi20_solid_r3_R2.fastq.gz
   
    ln -s ../X101SC26025981-Z01-J001/01.RawData/67/67_1.fq.gz AYE-T_Azi20_solid_r1_R1.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/67/67_2.fq.gz AYE-T_Azi20_solid_r1_R2.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/68/68_1.fq.gz AYE-T_Azi20_solid_r2_R1.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/68/68_2.fq.gz AYE-T_Azi20_solid_r2_R2.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/69/69_1.fq.gz AYE-T_Azi20_solid_r3_R1.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/69/69_2.fq.gz AYE-T_Azi20_solid_r3_R2.fastq.gz
   
    ln -s ../X101SC26025981-Z01-J001/01.RawData/64/64_1.fq.gz AYE-O_Azi20_solid_r1_R1.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/64/64_2.fq.gz AYE-O_Azi20_solid_r1_R2.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/65/65_1.fq.gz AYE-O_Azi20_solid_r2_R1.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/65/65_2.fq.gz AYE-O_Azi20_solid_r2_R2.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/66/66_1.fq.gz AYE-O_Azi20_solid_r3_R1.fastq.gz
    ln -s ../X101SC26025981-Z01-J001/01.RawData/66/66_2.fq.gz AYE-O_Azi20_solid_r3_R2.fastq.gz
   
    ln -s ../X101SC26025981-Z01-J001/01.RawData/70/70_1.fq.gz F_Azi20_solid_r1_R1.fastq.gz  #clinical
    ln -s ../X101SC26025981-Z01-J001/01.RawData/70/70_2.fq.gz F_Azi20_solid_r1_R2.fastq.gz  #clinical
    ln -s ../X101SC26025981-Z01-J001/01.RawData/71/71_1.fq.gz F_Azi20_solid_r2_R1.fastq.gz  #clinical
    ln -s ../X101SC26025981-Z01-J001/01.RawData/71/71_2.fq.gz F_Azi20_solid_r2_R2.fastq.gz  #clinical
    ln -s ../X101SC26025981-Z01-J001/01.RawData/72/72_1.fq.gz F_Azi20_solid_r3_R1.fastq.gz  #clinical
    ln -s ../X101SC26025981-Z01-J001/01.RawData/72/72_2.fq.gz F_Azi20_solid_r3_R2.fastq.gz  #clinical

2. Preparing the directory trimmed

    mkdir trimmed trimmed_unpaired;
    for sample_id in AYE-O_Azi20_solid_r1 AYE-O_Azi20_solid_r2 AYE-O_Azi20_solid_r3 AYE-O_ctr_r1 AYE-O_ctr_r2 AYE-O_ctr_r3 AYE-O_ctr_solid_r1 AYE-O_ctr_solid_r2 AYE-O_ctr_solid_r3 AYE-O_Diclo375_r1 AYE-O_Diclo375_r2 AYE-O_Diclo375_r3 AYE-O_Mero0.5_r1 AYE-O_Mero0.5_r2 AYE-O_Mero0.5_r3 AYE-O_Rifampicin2_r1 AYE-O_Rifampicin2_r2 AYE-O_Rifampicin2_r3 AYE-T_Azi20_solid_r1 AYE-T_Azi20_solid_r2 AYE-T_Azi20_solid_r3 AYE-T_ctr_r1 AYE-T_ctr_r2 AYE-T_ctr_r3 AYE-T_ctr_solid_r1 AYE-T_ctr_solid_r2 AYE-T_ctr_solid_r3 AYE-T_Diclo375_r1 AYE-T_Diclo375_r2 AYE-T_Diclo375_r3 AYE-T_Mero0.15_r1 AYE-T_Mero0.15_r2 AYE-T_Mero0.15_r3 AYE-T_Rifampicin2_r1 AYE-T_Rifampicin2_r2 AYE-T_Rifampicin2_r3 AYE-WT_Azi20_solid_r1 AYE-WT_Azi20_solid_r2 AYE-WT_Azi20_solid_r3 AYE-WT_ctr_r1 AYE-WT_ctr_r2 AYE-WT_ctr_r3 AYE-WT_ctr_solid_r1 AYE-WT_ctr_solid_r2 AYE-WT_ctr_solid_r3 AYE-WT_Diclo1250_solid_r1 AYE-WT_Diclo1250_solid_r2 AYE-WT_Diclo1250_solid_r3 AYE-WT_Diclo750_r1 AYE-WT_Diclo750_r2 AYE-WT_Diclo750_r3 AYE-WT_Mero0.35-0.5_r1 AYE-WT_Mero0.35-0.5_r2 AYE-WT_Mero0.35-0.5_r3 AYE-WT_Rifampicin1.5_r1 AYE-WT_Rifampicin1.5_r2 AYE-WT_Rifampicin1.5_r3 F_Azi20_solid_r1 F_Azi20_solid_r2 F_Azi20_solid_r3 F_ctr_solid_r1 F_ctr_solid_r2 F_ctr_solid_r3 O-Trans_ctr_r1 O-Trans_ctr_r2 O-Trans_ctr_r3 O-Trans_Diclo375_r1 O-Trans_Diclo375_r2 O-Trans_Diclo375_r3 O-Trans_Mero0.25_r1 O-Trans_Mero0.25_r2 O-Trans_Mero0.25_r3 O-Trans_Rifampicin2_r1 O-Trans_Rifampicin2_r2 O-Trans_Rifampicin2_r3 WT-Trans_ctr_r1 WT-Trans_ctr_r2 WT-Trans_ctr_r3 WT-Trans_Diclo750_r1 WT-Trans_Diclo750_r2 WT-Trans_Diclo750_r3; do \
    for sample_id in AYE-T_Diclo375_r2; do \
            java -jar /home/jhuang/Tools/Trimmomatic-0.36/trimmomatic-0.36.jar PE -threads 100 raw_data/${sample_id}_R1.fastq.gz raw_data/${sample_id}_R2.fastq.gz trimmed/${sample_id}_R1.fastq.gz trimmed_unpaired/${sample_id}_R1.fastq.gz trimmed/${sample_id}_R2.fastq.gz trimmed_unpaired/${sample_id}_R2.fastq.gz ILLUMINACLIP:/home/jhuang/Tools/Trimmomatic-0.36/adapters/TruSeq3-PE-2.fa:2:30:10:8:TRUE LEADING:3 TRAILING:3 SLIDINGWINDOW:4:15 MINLEN:36 AVGQUAL:20; done 2> trimmomatic_pe.log;
    done

3. (Optional) using trinity to find the most closely reference

    #Trinity --seqType fq --max_memory 50G --left trimmed/wt_r1_R1.fastq.gz  --right trimmed/wt_r1_R2.fastq.gz --CPU 12
   
    #https://www.genome.jp/kegg/tables/br08606.html#prok
    acb     KGB     Acinetobacter baumannii ATCC 17978  2007    GenBank
    abm     KGB     Acinetobacter baumannii SDF     2008    GenBank
    aby     KGB     Acinetobacter baumannii AYE     2008    GenBank --> *
    abc     KGB     Acinetobacter baumannii ACICU   2008    GenBank
    abn     KGB     Acinetobacter baumannii AB0057  2008    GenBank
    abb     KGB     Acinetobacter baumannii AB307-0294  2008    GenBank
    abx     KGB     Acinetobacter baumannii 1656-2  2012    GenBank
    abz     KGB     Acinetobacter baumannii MDR-ZJ06    2012    GenBank
    abr     KGB     Acinetobacter baumannii MDR-TJ  2012    GenBank
    abd     KGB     Acinetobacter baumannii TCDC-AB0715     2012    GenBank
    abh     KGB     Acinetobacter baumannii TYTH-1  2012    GenBank
    abad    KGB     Acinetobacter baumannii D1279779    2013    GenBank
    abj     KGB     Acinetobacter baumannii BJAB07104   2013    GenBank
    abab    KGB     Acinetobacter baumannii BJAB0715    2013    GenBank
    abaj    KGB     Acinetobacter baumannii BJAB0868    2013    GenBank
    abaz    KGB     Acinetobacter baumannii ZW85-1  2013    GenBank
    abk     KGB     Acinetobacter baumannii AbH12O-A2   2014    GenBank
    abau    KGB     Acinetobacter baumannii AB030   2014    GenBank
    abaa    KGB     Acinetobacter baumannii AB031   2014    GenBank
    abw     KGB     Acinetobacter baumannii AC29    2014    GenBank
    abal    KGB     Acinetobacter baumannii LAC-4   2015    GenBank
    #Note that the Acinetobacter baumannii strain ATCC 19606 chromosome, complete genome (GenBank: CU459141.1) was choosen as reference!

4. Preparing samplesheet.csv

    sample,fastq_1,fastq_2,strandedness
    Urine_r1,Urine_r1_R1.fq.gz,Urine_r1_R2.fq.gz,auto
    ...

5. Downloading CU459141.fasta and CU459141.gff from GenBank and preparing CU459141_m.gff

    #Example1: http://xgenes.com/article/article-content/157/prepare-virus-gtf-for-nextflow-run/
    #Default NOT_WORKING: --gtf_group_features 'gene_id'  --gtf_extra_attributes 'gene_name' --featurecounts_group_type 'gene_biotype' --featurecounts_feature_type 'exon'
    #(host_env) !NOT_WORKING! jhuang@WS-2290C:~/DATA/Data_Tam_RNAseq_2024$ /usr/local/bin/nextflow run rnaseq/main.nf --input samplesheet.csv --outdir results    --fasta "/home/jhuang/DATA/Data_Tam_RNAseq_2024/CU459141.fasta" --gff "/home/jhuang/DATA/Data_Tam_RNAseq_2024/CU459141.gff"        -profile docker -resume  --max_cpus 55 --max_memory 512.GB --max_time 2400.h    --save_align_intermeds --save_unaligned --save_reference    --aligner 'star_salmon'    --gtf_group_features 'gene_id'  --gtf_extra_attributes 'gene_name' --featurecounts_group_type 'gene_biotype' --featurecounts_feature_type 'transcript'
   
    # -- DEBUG_1 (CDS --> exon in CP059040.gff) --
    #Checking the record (see below) in results/genome/CP059040.gtf
    #In ./results/genome/CP059040.gtf e.g. "CP059040.1      Genbank transcript      1       1398    .       +       .       transcript_id "gene-H0N29_00005"; gene_id "gene-H0N29_00005"; gene_name "dnaA"; Name "dnaA"; gbkey "Gene"; gene "dnaA"; gene_biotype "protein_coding"; locus_tag "H0N29_00005";"
    #--featurecounts_feature_type 'transcript' returns only the tRNA results
    #Since the tRNA records have "transcript and exon". In gene records, we have "transcript and CDS". replace the CDS with exon
   
    grep -P "\texon\t" CP059040.gff | sort | wc -l    #96
    grep -P "cmsearch\texon\t" CP059040.gff | wc -l    #=10  ignal recognition particle sRNA small typ, transfer-messenger RNA, 5S ribosomal RNA
    grep -P "Genbank\texon\t" CP059040.gff | wc -l    #=12  16S and 23S ribosomal RNA
    grep -P "tRNAscan-SE\texon\t" CP059040.gff | wc -l    #tRNA 74
    wc -l star_salmon/AUM_r3/quant.genes.sf  #--featurecounts_feature_type 'transcript' results in 96 records!
   
    grep -P "\tCDS\t" CU459141.gff3 | wc -l  #3659
    sed 's/\tCDS\t/\texon\t/g' CU459141.gff3 > CU459141_m.gff
    grep -P "\texon\t" CU459141_m.gff | sort | wc -l  #3760
   
    # -- DEBUG_2: combination of 'CU459141_m.gff' and 'exon' results in ERROR, using 'transcript' instead!
    --gff "/home/jhuang/DATA/Data_Tam_RNAseq_2026_on_AYE/CU459141_m.gff" --featurecounts_feature_type 'transcript'
   
    # -- DEBUG_3: make sure the header of fasta is the same to the *_m.gff file

6. nextflow run

    # ---- SUCCESSFUL with directly downloaded gff3 and fasta from NCBI using docker after replacing 'CDS' with 'exon' ----
    (host_env) mv trimmed/*.fastq.gz .
    (host_env) nextflow run nf-core/rnaseq -r 3.14.0 -profile docker \

   –input samplesheet.csv –outdir results –fasta “/home/jhuang/DATA/Data_Tam_RNAseq_2026_on_AYE/CU459141.fasta” –gff “/home/jhuang/DATA/Data_Tam_RNAseq_2026_on_AYE/CU459141_m.gff” -resume –max_cpus 90 –max_memory 900.GB –max_time 2400.h –save_align_intermeds –save_unaligned –save_reference –aligner ‘star_salmon’ –gtf_group_features ‘gene_id’ –gtf_extra_attributes ‘gene_name’ –featurecounts_group_type ‘gene_biotype’ –featurecounts_feature_type ‘transcript’

7. Import data and pca-plot

    #TODO_AFTERNOON: at least sent today a PCA, am besten all comparison tables!
   
    #mamba activate r_env
   
    #install.packages("ggfun")
    # Import the required libraries
    library("AnnotationDbi")
    library("clusterProfiler")
    library("ReactomePA")
    library(gplots)
    library(tximport)
    library(DESeq2)
    #library("org.Hs.eg.db")
    library(dplyr)
    library(tidyverse)
    #install.packages("devtools")
    #devtools::install_version("gtable", version = "0.3.0")
    library(gplots)
    library("RColorBrewer")
    #install.packages("ggrepel")
    library("ggrepel")
    # install.packages("openxlsx")
    library(openxlsx)
    library(EnhancedVolcano)
    library(DESeq2)
    library(edgeR)
   
    setwd("~/DATA/Data_Tam_RNAseq_2026_on_AYE/results/star_salmon")
    # Define paths to your Salmon output quantification files
   
    # Store sample names in a character vector
    samples <- c(
        "AYE-O_Azi20_solid_r1", "AYE-O_Azi20_solid_r2", "AYE-O_Azi20_solid_r3", "AYE-O_ctr_r1", "AYE-O_ctr_r2",
        "AYE-O_ctr_r3", "AYE-O_ctr_solid_r1", "AYE-O_ctr_solid_r2", "AYE-O_ctr_solid_r3",
        "AYE-O_Diclo375_r1", "AYE-O_Diclo375_r2", "AYE-O_Diclo375_r3", "AYE-O_Mero0.5_r1",
        "AYE-O_Mero0.5_r2", "AYE-O_Mero0.5_r3", "AYE-O_Rifampicin2_r1", "AYE-O_Rifampicin2_r2",
        "AYE-O_Rifampicin2_r3", "AYE-T_Azi20_solid_r1", "AYE-T_Azi20_solid_r2", "AYE-T_Azi20_solid_r3",
        "AYE-T_ctr_r1", "AYE-T_ctr_r2", "AYE-T_ctr_r3", "AYE-T_ctr_solid_r1", "AYE-T_ctr_solid_r2",
        "AYE-T_ctr_solid_r3", "AYE-T_Diclo375_r1", "AYE-T_Diclo375_r2", "AYE-T_Diclo375_r3",
        "AYE-T_Mero0.15_r1", "AYE-T_Mero0.15_r2", "AYE-T_Mero0.15_r3", "AYE-T_Rifampicin2_r1",
        "AYE-T_Rifampicin2_r2", "AYE-T_Rifampicin2_r3", "AYE-WT_Azi20_solid_r1", "AYE-WT_Azi20_solid_r2",
        "AYE-WT_Azi20_solid_r3", "AYE-WT_ctr_r1", "AYE-WT_ctr_r2", "AYE-WT_ctr_r3", "AYE-WT_ctr_solid_r1",
        "AYE-WT_ctr_solid_r2", "AYE-WT_ctr_solid_r3", "AYE-WT_Diclo1250_solid_r1", "AYE-WT_Diclo1250_solid_r2",
        "AYE-WT_Diclo1250_solid_r3", "AYE-WT_Diclo750_r1", "AYE-WT_Diclo750_r2", "AYE-WT_Diclo750_r3",
        "AYE-WT_Mero0.35-0.5_r1", "AYE-WT_Mero0.35-0.5_r2", "AYE-WT_Mero0.35-0.5_r3", "AYE-WT_Rifampicin1.5_r1",
        "AYE-WT_Rifampicin1.5_r2", "AYE-WT_Rifampicin1.5_r3", "F_Azi20_solid_r1", "F_Azi20_solid_r2",
        "F_Azi20_solid_r3", "F_ctr_solid_r1", "F_ctr_solid_r2", "F_ctr_solid_r3", "O-Trans_ctr_r1",
        "O-Trans_ctr_r2", "O-Trans_ctr_r3", "O-Trans_Diclo375_r1", "O-Trans_Diclo375_r2", "O-Trans_Diclo375_r3",
        "O-Trans_Mero0.25_r1", "O-Trans_Mero0.25_r2", "O-Trans_Mero0.25_r3", "O-Trans_Rifampicin2_r1",
        "O-Trans_Rifampicin2_r2", "O-Trans_Rifampicin2_r3", "WT-Trans_ctr_r1", "WT-Trans_ctr_r2",
        "WT-Trans_ctr_r3", "WT-Trans_Diclo750_r1", "WT-Trans_Diclo750_r2", "WT-Trans_Diclo750_r3"
    )
   
    ## Automatically generate the named vector
    files <- setNames(paste0("./", samples, "/quant.sf"), samples)
   
    # -----------------------------------------------------------------
    # ---- Step 1: Create Detailed Metadata from Your Sample Names ----
   
    # Extract metadata from sample names
    samples <- names(files)
   
    # Parse the complex sample names
    metadata <- data.frame(
    sample = samples,
    stringsAsFactors = FALSE
    )
   
    # Extract strain (everything before first underscore or hyphen treatment)
    metadata$strain <- sapply(strsplit(samples, "[-_]"), function(x) {
    if(x[1] %in% c("AYE", "O", "WT", "F")) {
        if(x[1] == "AYE" && length(x) > 1 && x[2] %in% c("WT", "T", "O")) {
        paste(x[1:2], collapse = "-")
        } else if(x[1] %in% c("O", "WT") && x[2] == "Trans") {
        paste(x[1:2], collapse = "-")
        } else {
        x[1]
        }
    } else {
        x[1]
    }
    })
   
    # Extract treatment type
    metadata$treatment <- sapply(samples, function(x) {
    if(grepl("_ctr", x)) return("ctrl")
    if(grepl("Diclo", x)) return("Diclo")
    if(grepl("Mero", x)) return("Mero")
    if(grepl("Azi", x)) return("Azi")
    if(grepl("Rifampicin", x)) return("Rifampicin")
    return("ctrl")
    })
   
    # Extract concentration
    metadata$concentration <- sapply(samples, function(x) {
    if(grepl("Diclo1250", x)) return("1250")
    if(grepl("Diclo750", x)) return("750")
    if(grepl("Diclo375", x)) return("375")
    if(grepl("Mero0.5", x)) return("0.5")
    if(grepl("Mero0.35", x)) return("0.35")
    if(grepl("Mero0.25", x)) return("0.25")
    if(grepl("Mero0.15", x)) return("0.15")
    if(grepl("Azi20", x)) return("20")
    if(grepl("Rifampicin2", x)) return("2")
    if(grepl("Rifampicin1.5", x)) return("1.5")
    return("0")
    })
   
    # Extract condition (solid vs liquid)
    metadata$condition <- ifelse(grepl("_solid", samples), "solid", "liquid")
   
    # Extract replicate
    metadata$replicate <- sapply(strsplit(samples, "_"), function(x) {
    rep_part <- x[length(x)]
    gsub("r", "", rep_part)
    })
   
    # Create combined group for easy comparisons
    metadata$group <- paste(metadata$strain, metadata$treatment, metadata$concentration, sep = "_")
   
    # Set row names
    rownames(metadata) <- metadata$sample
   
    # Reorder to match txi columns
    metadata <- metadata[colnames(txi$counts), ]
   
    # ---------------------------------------------
    # ---- Step 2: Choose Your Design Strategy ----
   
    # Strategy A: Full Factorial Design (if balanced)
    dds <- DESeqDataSetFromTximport(txi, metadata,
                             design = ~ strain + treatment + condition)
   
    # --> Strategy B: Combined Group Factor ⭐ RECOMMENDED
    metadata$group <- factor(paste(metadata$strain,
                                    metadata$treatment,
                                    metadata$concentration,
                                    metadata$condition,
                                    sep = "_"))
   
    dds <- DESeqDataSetFromTximport(txi, metadata,
                                    design = ~ group)
    dds <- DESeq(dds)
   
    # See all available comparisons
    resultsNames(dds)
   
    # -------------------------------------------------------------
    # ---- Step 3: Set Up Specific Comparisons from Your Notes ----
    # ==========================================
    # 1. Define Exact Comparisons from Your Notes
    # ==========================================
    planned_comparisons <- list(
    # --- Baseline / Strain Controls ---
    AYE_T_ctr_vs_AYE_WT_ctr            = list(treat = "AYE-T_ctrl_0_liquid",   ctrl = "AYE-WT_ctrl_0_liquid"),
    AYE_O_ctr_vs_AYE_WT_ctr            = list(treat = "AYE-O_ctrl_0_liquid",   ctrl = "AYE-WT_ctrl_0_liquid"),
    O_Trans_ctr_vs_AYE_WT_ctr          = list(treat = "O-Trans_ctrl_0_liquid", ctrl = "AYE-WT_ctrl_0_liquid"),
    WT_Trans_ctr_vs_AYE_WT_ctr         = list(treat = "WT-Trans_ctrl_0_liquid",ctrl = "AYE-WT_ctrl_0_liquid"),
    AYE_O_ctr_vs_AYE_T                 = list(treat = "AYE-O_ctrl_0_liquid",   ctrl = "AYE-T_ctrl_0_liquid"),
    O_Trans_ctr_vs_AYE_T               = list(treat = "O-Trans_ctrl_0_liquid", ctrl = "AYE-T_ctrl_0_liquid"),
    WT_Trans_ctr_vs_AYE_T              = list(treat = "WT-Trans_ctrl_0_liquid",ctrl = "AYE-T_ctrl_0_liquid"),
   
    # --- Condition Effects (Solid vs Liquid) ---
    AYE_WT_ctr_solid_vs_AYE_WT_ctr     = list(treat = "AYE-WT_ctrl_0_solid",   ctrl = "AYE-WT_ctrl_0_liquid"),
    AYE_O_ctr_solid_vs_AYE_O_ctr       = list(treat = "AYE-O_ctrl_0_solid",    ctrl = "AYE-O_ctrl_0_liquid"),
    AYE_T_ctr_solid_vs_AYE_T_ctr       = list(treat = "AYE-T_ctrl_0_solid",    ctrl = "AYE-T_ctrl_0_liquid"),
    AYE_O_ctr_solid_vs_AYE_WT_ctr_solid= list(treat = "AYE-O_ctrl_0_solid",    ctrl = "AYE-WT_ctrl_0_solid"),
    AYE_T_ctr_solid_vs_AYE_WT_ctr_solid= list(treat = "AYE-T_ctrl_0_solid",    ctrl = "AYE-WT_ctrl_0_solid"),
   
    # --- Diclofenac ---
    AYE_WT_Diclo750_vs_AYE_WT_ctr      = list(treat = "AYE-WT_Diclo_750_liquid",   ctrl = "AYE-WT_ctrl_0_liquid"),
    AYE_T_Diclo375_vs_AYE_WT_ctr       = list(treat = "AYE-T_Diclo_375_liquid",    ctrl = "AYE-WT_ctrl_0_liquid"),
    AYE_O_Diclo375_vs_AYE_WT_ctr       = list(treat = "AYE-O_Diclo_375_liquid",    ctrl = "AYE-WT_ctrl_0_liquid"),
    O_Trans_Diclo375_vs_AYE_WT_ctr     = list(treat = "O-Trans_Diclo_375_liquid",  ctrl = "AYE-WT_ctrl_0_liquid"),
    WT_Trans_Diclo750_vs_AYE_WT_ctr    = list(treat = "WT-Trans_Diclo_750_liquid", ctrl = "AYE-WT_ctrl_0_liquid"),
    Diclo_AYE_WT_1250_solid_vs_solid_ctr = list(treat = "AYE-WT_Diclo_1250_solid", ctrl = "AYE-WT_ctrl_0_solid"),
   
    # --- Meropenem ---
    AYE_WT_Mero_vs_AYE_WT_ctr          = list(treat = "AYE-WT_Mero_0.35_liquid", ctrl = "AYE-WT_ctrl_0_liquid"),
    AYE_T_Mero_vs_AYE_WT_ctr           = list(treat = "AYE-T_Mero_0.15_liquid",      ctrl = "AYE-WT_ctrl_0_liquid"),
    AYE_O_Mero_vs_AYE_WT_ctr           = list(treat = "AYE-O_Mero_0.5_liquid",       ctrl = "AYE-WT_ctrl_0_liquid"),
    O_Trans_Mero_vs_AYE_WT_ctr         = list(treat = "O-Trans_Mero_0.25_liquid",    ctrl = "AYE-WT_ctrl_0_liquid"),
    AYE_T_Mero_vs_AYE_T_ctr            = list(treat = "AYE-T_Mero_0.15_liquid",      ctrl = "AYE-T_ctrl_0_liquid"),
   
    # --- Azithromycin (Solid) ---
    AYE_WT_Azi_vs_solid_ctr            = list(treat = "AYE-WT_Azi_20_solid", ctrl = "AYE-WT_ctrl_0_solid"),
    AYE_T_Azi_vs_solid_ctr             = list(treat = "AYE-T_Azi_20_solid",  ctrl = "AYE-T_ctrl_0_solid"),
    AYE_O_Azi_vs_solid_ctr             = list(treat = "AYE-O_Azi_20_solid",  ctrl = "AYE-O_ctrl_0_solid"),
    F_Azi_vs_F_solid_ctr               = list(treat = "F_Azi_20_solid",      ctrl = "F_ctrl_0_solid"),
   
    # --- Rifampicin ---
    AYE_WT_Rif_vs_AYE_WT_ctr           = list(treat = "AYE-WT_Rifampicin_1.5_liquid", ctrl = "AYE-WT_ctrl_0_liquid"),
    AYE_T_Rif_vs_AYE_T_ctr             = list(treat = "AYE-T_Rifampicin_2_liquid",    ctrl = "AYE-T_ctrl_0_liquid"),
    AYE_O_Rif_vs_AYE_O_ctr             = list(treat = "AYE-O_Rifampicin_2_liquid",    ctrl = "AYE-O_ctrl_0_liquid"),
    O_Trans_Rif_vs_O_Trans_ctr         = list(treat = "O-Trans_Rifampicin_2_liquid",  ctrl = "O-Trans_ctrl_0_liquid")
    )
   
    # ==========================================
    # 2. Verification & Validation Script
    # ==========================================
    # Identify which column in colData holds your group names
    group_col <- if("group" %in% colnames(colData(dds))) "group" else
                if("treatment" %in% colnames(colData(dds))) "treatment" else
                stop("❌ Please specify the correct colData column containing group names.")
   
    actual_groups <- unique(colData(dds)[[group_col]])
   
    cat("\n", paste(rep("=", 85), collapse=""), "\n")
    cat("📋 VERIFICATION OF NOTE-DERIVED COMPARISONS\n")
    cat(paste(rep("=", 85), collapse=""), "\n\n")
   
    validation_results <- data.frame(
    Comparison_Name = character(),
    Treatment_String = character(),
    Control_String = character(),
    Status = character(),
    Suggested_Contrast = character(),
    stringsAsFactors = FALSE
    )
   
    for(name in names(planned_comparisons)) {
    trt <- planned_comparisons[[name]]$treat
    ctl <- planned_comparisons[[name]]$ctrl
   
    # Find closest matches in actual data
    trt_match <- actual_groups[grepl(trt, actual_groups, fixed = TRUE)]
    ctl_match <- actual_groups[grepl(ctl, actual_groups, fixed = TRUE)]
   
    status <- if(length(trt_match) > 0 && length(ctl_match) > 0) "✅ VALID" else "⚠️  CHECK"
    contrast_str <- if(status == "✅ VALID")
        paste0('c("', group_col, '", "', trt_match[1], '", "', ctl_match[1], '")') else "N/A"
   
    validation_results <- rbind(validation_results, data.frame(
        Comparison_Name = name,
        Treatment_String = trt,
        Control_String = ctl,
        Status = status,
        Suggested_Contrast = contrast_str,
        stringsAsFactors = FALSE
    ))
   
    cat(sprintf("%-45s | T:%-25s C:%-20s | %s\n", name, trt, ctl, status))
    if(status == "⚠️  CHECK") {
        if(length(trt_match) == 0) cat("   🔍 Treat not found. Closest: ", paste(head(actual_groups[grepl(strsplit(trt, "_")[[1]][1], actual_groups)], 3), collapse=", "), "\n")
        if(length(ctl_match) == 0) cat("   🔍 Ctrl not found.  Closest: ", paste(head(actual_groups[grepl(strsplit(ctl, "_")[[1]][1], actual_groups)], 3), collapse=", "), "\n")
    }
    }
   
    # ==========================================
    # 3. Auto-Generate DESeq2 results() Calls (Optional)
    # ==========================================
    valid_comparisons <- validation_results[validation_results$Status == "✅ VALID", ]
    if(nrow(valid_comparisons) > 0) {
    cat("\n📜 READY-TO-RUN DESeq2 CONTRASTS:\n")
    cat(paste(rep("-", 60), collapse=""), "\n")
    for(i in seq_len(nrow(valid_comparisons))) {
        cat(sprintf('res_%s <- results(dds, contrast = %s)\n',
                    gsub("[^A-Za-z0-9]", "_", valid_comparisons$Comparison_Name[i]),
                    valid_comparisons$Suggested_Contrast[i]))
    }
    } else {
    cat("\n⚠️  No exact matches found. Check your colData group naming convention.\n")
    }
   
    # -----------------------------
    # ---- Step 4: PCA figures ----
   
    # 🔍 What each figure shows:
    #
    #    01_PCA_by_Strain.png → Tests if genetic background (AYE-WT, AYE-T, AYE-O, Trans, F) is the dominant source of variation.
    #    02_PCA_by_Treatment.png → Shows clustering by antibiotic/drug exposure (ctrl, Diclo, Mero, Azi, Rifampicin).
    #    03_PCA_by_Condition.png → Reveals batch/growth media effects (solid vs liquid).
    #    04_PCA_CombinedGroups.png → Full experimental grouping with labeled sample names for quick outlier detection.
    #    05_PCA_Ellipses.png → Adds 95% confidence boundaries per strain to visualize group spread and overlap.
    #
    # ⚠️ Quick Checklist Before Running:
    #
    #    Ensure metadata columns (strain, treatment, condition, group) are attached to colData(dds).
    #    If ggrepel is missing, run install.packages("ggrepel").
    #    All PNGs will save to your current working directory (getwd()).
   
    # Install if missing: install.packages(c("ggplot2", "ggrepel"))
    library(DESeq2)
    library(ggplot2)
    library(ggrepel)
   
    # 1. Variance Stabilizing Transformation & Extract PCA Data
    vsd <- vst(dds, blind = FALSE)
    pca_data <- plotPCA(vsd, intgroup = c("strain", "treatment", "condition", "group"), returnData = TRUE)
    percent_var <- round(100 * attr(pca_data, "percentVar"))
   
    # Consistent theme for all plots
    base_theme <- theme_bw(base_size = 12) +
    theme(plot.title = element_text(hjust = 0.5, face = "bold", size = 13),
            legend.position = "right",
            legend.title = element_text(face = "bold"),
            panel.grid.major = element_line(color = "grey90"),
            panel.grid.minor = element_blank())
   
    # --- Plot 1: Colored by Strain ---
    p1 <- ggplot(pca_data, aes(x = PC1, y = PC2, color = strain, shape = condition)) +
    geom_point(size = 3, alpha = 0.8) +
    geom_text_repel(aes(label = name), size = 2.5, max.overlaps = 20, show.legend = FALSE) +
    labs(x = paste0("PC1: ", percent_var[1], "% variance"),
        y = paste0("PC2: ", percent_var[2], "% variance"),
        title = "PCA: Samples Colored by Strain",
        color = "Strain", shape = "Condition") +
    base_theme
    ggsave("01_PCA_by_Strain.png", p1, width = 8, height = 6, dpi = 300)
   
    # --- Plot 2: Colored by Treatment ---
    p2 <- ggplot(pca_data, aes(x = PC1, y = PC2, color = treatment, shape = condition)) +
    geom_point(size = 3, alpha = 0.8) +
    labs(x = paste0("PC1: ", percent_var[1], "% variance"),
        y = paste0("PC2: ", percent_var[2], "% variance"),
        title = "PCA: Samples Colored by Treatment",
        color = "Treatment", shape = "Condition") +
    base_theme
    ggsave("02_PCA_by_Treatment.png", p2, width = 8, height = 6, dpi = 300)
   
    # --- Plot 3: Colored by Condition (Solid vs Liquid) ---
    p3 <- ggplot(pca_data, aes(x = PC1, y = PC2, color = condition, shape = strain)) +
    geom_point(size = 3, alpha = 0.8) +
    labs(x = paste0("PC1: ", percent_var[1], "% variance"),
        y = paste0("PC2: ", percent_var[2], "% variance"),
        title = "PCA: Samples Colored by Growth Condition",
        color = "Condition", shape = "Strain") +
    base_theme
    ggsave("03_PCA_by_Condition.png", p3, width = 8, height = 6, dpi = 300)
   
    # --- Plot 4: Combined Groups with Sample Labels ---
    p4 <- ggplot(pca_data, aes(x = PC1, y = PC2, color = group)) +
    geom_point(size = 3, alpha = 0.8) +
    geom_text_repel(aes(label = name), size = 2, max.overlaps = 30, box.padding = 0.3) +
    labs(x = paste0("PC1: ", percent_var[1], "% variance"),
        y = paste0("PC2: ", percent_var[2], "% variance"),
        title = "PCA: Combined Experimental Groups",
        color = "Group") +
    base_theme + theme(legend.position = "none")
    ggsave("04_PCA_CombinedGroups.png", p4, width = 9, height = 7, dpi = 300)
   
    # --- Plot 5: 95% Confidence Ellipses (by Strain) ---
    p5 <- ggplot(pca_data, aes(x = PC1, y = PC2, color = strain, fill = strain)) +
    geom_point(size = 3, alpha = 0.7) +
    stat_ellipse(level = 0.95, alpha = 0.2, geom = "polygon", show.legend = FALSE) +
    labs(x = paste0("PC1: ", percent_var[1], "% variance"),
        y = paste0("PC2: ", percent_var[2], "% variance"),
        title = "PCA: 95% Confidence Ellipses by Strain",
        color = "Strain", fill = "Strain") +
    base_theme
    ggsave("05_PCA_Ellipses.png", p5, width = 8, height = 6, dpi = 300)
   
    message("✅ All 5 PCA plots saved to working directory!")

8. Run Differential Expression & PCA Analysis Complete

    (r_env) jhuang@WS-2290C:/mnt/md1/DATA/Data_Tam_RNAseq_2026_on_AYE/results/star_salmon$ Rscript complete_deg_pipeline.R

variant_annot_2026__final.xls

1. Input data:

    # ---- Datasets 2024 (in total 4) ----
    ln -s ../../Data_Pietschmann_229ECoronavirus_Mutations_2025/raw_data_2024/hCoV229E_Rluc_R1.fastq.gz hCoV229E_Rluc_R1.fastq.gz
    ln -s ../../Data_Pietschmann_229ECoronavirus_Mutations_2025/raw_data_2024/hCoV229E_Rluc_R2.fastq.gz hCoV229E_Rluc_R2.fastq.gz
    ln -s ../../Data_Pietschmann_229ECoronavirus_Mutations_2025/raw_data_2024/p10_DMSO_R1.fastq.gz DMSO_p10_R1.fastq.gz
    ln -s ../../Data_Pietschmann_229ECoronavirus_Mutations_2025/raw_data_2024/p10_DMSO_R2.fastq.gz DMSO_p10_R2.fastq.gz
    ln -s ../../Data_Pietschmann_229ECoronavirus_Mutations_2025/raw_data_2024/p10_K22_R1.fastq.gz K22_p10_R1.fastq.gz
    ln -s ../../Data_Pietschmann_229ECoronavirus_Mutations_2025/raw_data_2024/p10_K22_R2.fastq.gz K22_p10_R2.fastq.gz
    ln -s ../../Data_Pietschmann_229ECoronavirus_Mutations_2025/raw_data_2024/p10_K7523_R1.fastq.gz X7523_p10_R1.fastq.gz
    ln -s ../../Data_Pietschmann_229ECoronavirus_Mutations_2025/raw_data_2024/p10_K7523_R2.fastq.gz X7523_p10_R2.fastq.gz
   
    # ---- Datasets 2025 (in total 3) ----
    ln -s ../../Data_Pietschmann_229ECoronavirus_Mutations_2025/raw_data_2025/250506_VH00358_136_AAG3YJ5M5/p20606/p16_DMSO_S29_R1_001.fastq.gz DMSO_p16_R1.fastq.gz
    ln -s ../../Data_Pietschmann_229ECoronavirus_Mutations_2025/raw_data_2025/250506_VH00358_136_AAG3YJ5M5/p20606/p16_DMSO_S29_R2_001.fastq.gz DMSO_p16_R2.fastq.gz
    ln -s ../../Data_Pietschmann_229ECoronavirus_Mutations_2025/raw_data_2025/250506_VH00358_136_AAG3YJ5M5/p20607/p16_K22_S30_R1_001.fastq.gz K22_p16_R1.fastq.gz
    ln -s ../../Data_Pietschmann_229ECoronavirus_Mutations_2025/raw_data_2025/250506_VH00358_136_AAG3YJ5M5/p20607/p16_K22_S30_R2_001.fastq.gz K22_p16_R2.fastq.gz
    ln -s ../../Data_Pietschmann_229ECoronavirus_Mutations_2025/raw_data_2025/250506_VH00358_136_AAG3YJ5M5/p20608/p16_X7523_S31_R1_001.fastq.gz X7523_p16_R1.fastq.gz
    ln -s ../../Data_Pietschmann_229ECoronavirus_Mutations_2025/raw_data_2025/250506_VH00358_136_AAG3YJ5M5/p20608/p16_X7523_S31_R2_001.fastq.gz X7523_p16_R2.fastq.gz
   
    # ---- Datasets 2026 (in total 3) ----
    ln -s ../raw_data_2026/20260212_AV243904_0054_B/02_DMSO_p26/02_DMSO_p26_R1.fastq.gz DMSO_p26_R1.fastq.gz
    ln -s ../raw_data_2026/20260212_AV243904_0054_B/02_DMSO_p26/02_DMSO_p26_R2.fastq.gz DMSO_p26_R2.fastq.gz
    ln -s ../raw_data_2026/20260212_AV243904_0054_B/01_K22_p26/01_K22_p26_R1.fastq.gz K22_p26_R1.fastq.gz
    ln -s ../raw_data_2026/20260212_AV243904_0054_B/01_K22_p26/01_K22_p26_R2.fastq.gz K22_p26_R2.fastq.gz
    ln -s ../raw_data_2026/20260212_AV243904_0054_B/03_X723_p26/03_X723_p26_R1.fastq.gz X7523_p26_R1.fastq.gz
    ln -s ../raw_data_2026/20260212_AV243904_0054_B/03_X723_p26/03_X723_p26_R2.fastq.gz X7523_p26_R2.fastq.gz

2. Call variant calling using snippy

    ln -s ~/Tools/bacto/db/ .;
    ln -s ~/Tools/bacto/envs/ .;
    ln -s ~/Tools/bacto/local/ .;
    cp ~/Tools/bacto/Snakefile .;
    cp ~/Tools/bacto/bacto-0.1.json .;
    cp ~/Tools/bacto/cluster.json .;
   
    #download CU459141.gb from GenBank
    mv ~/Downloads/sequence\(2\).gb db/PP810610.gb
   
    #setting the following in bacto-0.1.json
        "fastqc": false,
        "taxonomic_classifier": false,
        "assembly": true,
        "typing_ariba": false,
        "typing_mlst": true,
        "pangenome": true,
        "variants_calling": true,
        "phylogeny_fasttree": true,
        "phylogeny_raxml": true,
        "recombination": false, (due to gubbins-error set false)
        "genus": "Alphacoronavirus",
        "kingdom": "Viruses",
        "species": "Human coronavirus 229E",
        "mykrobe": {
            "species": "corona"
        },
        "reference": "db/PP810610.gb"
   
    mamba activate /home/jhuang/miniconda3/envs/bengal3_ac3
    (bengal3_ac3) /home/jhuang/miniconda3/envs/snakemake_4_3_1/bin/snakemake --printshellcmds

3. Summarize all SNPs and Indels from the snippy result directory.

    cp ~/Scripts/summarize_snippy_res_ordered.py .
    # IMPORTANT_ADAPT the array isolates = ["hCoV229E_Rluc", "DMSO_p10", "K22_p10", "X7523_p10", "DMSO_p16", "K22_p16", "X7523_p16", "DMSO_p26", "K22_p26", "X7523_p26"]
    mamba activate plot-numpy1
    python3 ./summarize_snippy_res_ordered.py snippy
    #--> Summary CSV file created successfully at: snippy/summary_snps_indels.csv
    cd snippy
    #REMOVE_the_line? I don't find the sence of the line:    grep -v "None,,,,,,None,None" summary_snps_indels.csv > summary_snps_indels_.csv

4. Using spandx calling variants (almost the same results to the one from viral-ngs!)

    mamba deactivate
    mamba activate /home/jhuang/miniconda3/envs/spandx
    mkdir ~/miniconda3/envs/spandx/share/snpeff-5.1-2/data/PP810610
    cp PP810610.gb  ~/miniconda3/envs/spandx/share/snpeff-5.1-2/data/PP810610/genes.gbk
    vim ~/miniconda3/envs/spandx/share/snpeff-5.1-2/snpEff.config
    /home/jhuang/miniconda3/envs/spandx/bin/snpEff build PP810610    #-d
    ~/Scripts/genbank2fasta.py PP810610.gb
    mv PP810610.gb_converted.fna PP810610.fasta    #rename "NC_001348.1 xxxxx" to "NC_001348" in the fasta-file
    ln -s /home/jhuang/Tools/spandx/ spandx
    (spandx) nextflow run spandx/main.nf --fastq "trimmed/*_P_{1,2}.fastq" --ref PP810610.fasta --annotation --database PP810610 -resume
   
    # RERUN SNP_matrix.sh due to the error ERROR_CHROMOSOME_NOT_FOUND in the variants annotation --> IT WORKS!
    cd Outputs/Master_vcf
    conda activate /home/jhuang/miniconda3/envs/spandx
    (spandx) cp -r ../../snippy/hCoV229E_Rluc/reference .
    (spandx) cp ../../spandx/bin/SNP_matrix.sh ./
    #Note that ${variant_genome_path}=NC_001348 in the following command, but it was not used after the following command modification.
    #Adapt "snpEff eff -no-downstream -no-intergenic -ud 100 -formatEff -v ${variant_genome_path} out.vcf > out.annotated.vcf" to
    "/home/jhuang/miniconda3/envs/bengal3_ac3/bin/snpEff eff -no-downstream -no-intergenic -ud 100 -formatEff -c reference/snpeff.config -dataDir . ref out.vcf > out.annotated.vcf" in SNP_matrix.sh
    (spandx) bash SNP_matrix.sh PP810610 .

5. Calling inter-host variants by merging the results from snippy+spandx (Manually! Note that the sample order of two tools are different, we should reorder the SNP-columns of spandx-results.)

    # Inter-host variants（宿主间变异）:一种病毒在两个人之间有不同的基因变异，这些变异可能与宿主的免疫反应、疾病表现或病毒传播的方式相关。
    cp All_SNPs_indels_annotated.txt All_SNPs_indels_annotated_backup.txt
    vim All_SNPs_indels_annotated.txt
   
    #in the file ids: grep "$(echo -e '\t')353$(echo -e '\t')" All_SNPs_indels_annotated.txt >> All_SNPs_indels_annotated_.txt
    #Replace \n with " All_SNPs_indels_annotated.txt >> All_SNPs_indels_annotated_.txt\ngrep "
    #Replace grep " --> grep "$(echo -e '\t')
    #Replace " All_ --> $(echo -e '\t')" All_
   
    # Potential intra-host variants: 10871, 19289, 21027, 23435.
    CHROM   POS REF ALT TYPE    hCoV229E_Rluc   DMSO_p10    K22_p10 X7523_p10   DMSO_p16    K22_p16 X7523_p16   DMSO_p26    K22_p26 X7523_p26   Effect  Impact  Functional_Class    Codon_change    Protein_and_nucleotide_change   Amino_Acid_Length   Gene_name   Biotype
    PP810610    1464    T   C   SNP C   C   C   C   C   C   C   C   C   C   missense_variant    MODERATE    MISSENSE    gTt/gCt p.Val416Ala/c.1247T>C   6757    CDS_1   protein_coding
    PP810610    1492    T   A   SNP T/A T/A T/A T/A T/A T/A T/A T   T/A T/A synonymous_variant  LOW SILENT  acT/acA p.Thr425Thr/c.1275T>A   6757    CDS_1   protein_coding
    PP810610    1699    C   T   SNP T   T   T   T   T   T   T   T   T   T   synonymous_variant  LOW SILENT  gtC/gtT p.Val494Val/c.1482C>T   6757    CDS_1   protein_coding
    PP810610    4809    A   C   SNP A   A   A   A   A   A   A/C A   A   A/C missense_variant    MODERATE    MISSENSE    gAt/gCt p.Asp1531Ala/c.4592A>C  6757    CDS_1   protein_coding
    PP810610    6470    C   T   SNP C   C   C   C   C   C   C   C   C/T C   synonymous_variant  LOW SILENT  Ctg/Ttg p.Leu2085Leu/c.6253C>T  6757    CDS_1   protein_coding
    PP810610    6691    C   T   SNP T   T   T   T   T   T   T   T   T   T   synonymous_variant  LOW SILENT  tgC/tgT p.Cys2158Cys/c.6474C>T  6757    CDS_1   protein_coding
    PP810610    6919    C   G   SNP G   G   G   G   G   G   G   G   G   G   synonymous_variant  LOW SILENT  ggC/ggG p.Gly2234Gly/c.6702C>G  6757    CDS_1   protein_coding
    PP810610    7294    T   A   SNP A   A   A   A   A   A   A   A   A   A   missense_variant    MODERATE    MISSENSE    agT/agA p.Ser2359Arg/c.7077T>A  6757    CDS_1   protein_coding
    PP810610    8289    C   A   SNP C/A C/A C   C/A C   C   C/A C   C   C/A missense_variant    MODERATE    MISSENSE    gCc/gAc p.Ala2691Asp/c.8072C>A  6757    CDS_1   protein_coding
    PP810610    8294    A   G   SNP A/G A   A/G A   A   A/G A   A   A/G A   missense_variant    MODERATE    MISSENSE    Aaa/Gaa p.Lys2693Glu/c.8077A>G  6757    CDS_1   protein_coding
    PP810610    8376    G   T   SNP G/T G   G   G   G   G   G   G   G   G   missense_variant    MODERATE    MISSENSE    cGt/cTt p.Arg2720Leu/c.8159G>T  6757    CDS_1   protein_coding
    PP810610    9146    T   C   SNP T   T   T   T/C T   T   T/C T   T   T   missense_variant    MODERATE    MISSENSE    Ttt/Ctt p.Phe2977Leu/c.8929T>C  6757    CDS_1   protein_coding
    PP810610    9174    G   A   SNP G   G   G   G/A G   G   G/A G   G   G   missense_variant    MODERATE    MISSENSE    tGc/tAc p.Cys2986Tyr/c.8957G>A  6757    CDS_1   protein_coding
    PP810610    9261    C   T   SNP C   C   C   C   C   C   C   C   C/T C   missense_variant    MODERATE    MISSENSE    gCt/gTt p.Ala3015Val/c.9044C>T  6757    CDS_1   protein_coding
    PP810610    10145   A   G   SNP A   A   A   A/G A   A   A/G A   A   A/G missense_variant    MODERATE    MISSENSE    Atg/Gtg p.Met3310Val/c.9928A>G  6757    CDS_1   protein_coding
    PP810610    10239   T   G   SNP T   T   T/G T   T   T/G T   T   T   T   missense_variant    MODERATE    MISSENSE    gTg/gGg p.Val3341Gly/c.10022T>G 6757    CDS_1   protein_coding
    PP810610    10310   G   A   SNP G   G   G   G/A G   G   G/A G   G   G/A missense_variant    MODERATE    MISSENSE    Gtt/Att p.Val3365Ile/c.10093G>A 6757    CDS_1   protein_coding
    PP810610    10432   C   T   SNP C   C   C   C   C   C   C   C   C   C/T synonymous_variant  LOW SILENT  ttC/ttT p.Phe3405Phe/c.10215C>T 6757    CDS_1   protein_coding
    PP810610    10871   C   T   SNP C   C/T T   C/T C/T T   C/T C   T   C/T missense_variant    MODERATE    MISSENSE    Ctt/Ttt p.Leu3552Phe/c.10654C>T 6757    CDS_1   protein_coding
    PP810610    10898   G   A   SNP G   G/A G   G/A G   G   G/A G   G   G/A missense_variant    MODERATE    MISSENSE    Ggc/Agc p.Gly3561Ser/c.10681G>A 6757    CDS_1   protein_coding
    PP810610    11418   C   A   SNP C   C   C   C   C   C   C   C   C/A C   missense_variant    MODERATE    MISSENSE    aCt/aAt p.Thr3734Asn/c.11201C>A 6757    CDS_1   protein_coding
    PP810610    11577   A   C   SNP A   A/C A   A   A/C A   A   A/C A   A   missense_variant    MODERATE    MISSENSE    gAa/gCa p.Glu3787Ala/c.11360A>C 6757    CDS_1   protein_coding
    PP810610    14472   T   C   SNP C   C   C   C   C   C   C   C   C   C   missense_variant    MODERATE    MISSENSE    aTg/aCg p.Met4752Thr/c.14255T>C 6757    CDS_1   protein_coding
    PP810610    15270   G   A   SNP G   G   G   G   G   G   G   G   G   G/A missense_variant    MODERATE    MISSENSE    cGa/cAa p.Arg5018Gln/c.15053G>A 6757    CDS_1   protein_coding
    PP810610    15458   T   C   SNP C   C   C   C   C   C   C   C   C   C   synonymous_variant  LOW SILENT  Ttg/Ctg p.Leu5081Leu/c.15241T>C 6757    CDS_1   protein_coding
    PP810610    16035   C   A   SNP A   A   A   A   A   A   A   A   A   A   stop_gained HIGH    NONSENSE    tCa/tAa p.Ser5273*/c.15818C>A   6757    CDS_1   protein_coding
    PP810610    17119   A   G   SNP A   A   A   A   A   A   A   A   A   A/G synonymous_variant  LOW SILENT  aaA/aaG p.Lys5634Lys/c.16902A>G 6757    CDS_1   protein_coding
    PP810610    17430   T   C   SNP C   C   C   C   C   C   C   C   C   C   missense_variant    MODERATE    MISSENSE    tTa/tCa p.Leu5738Ser/c.17213T>C 6757    CDS_1   protein_coding
    PP810610    18640   T   G   SNP T   T   T   T/G T   T   T/G T   T   T/G missense_variant    MODERATE    MISSENSE    tgT/tgG p.Cys6141Trp/c.18423T>G 6757    CDS_1   protein_coding
    PP810610    18646   C   T   SNP C   C   C   C/T C   C   C   C   C   C   synonymous_variant  LOW SILENT  taC/taT p.Tyr6143Tyr/c.18429C>T 6757    CDS_1   protein_coding
    PP810610    18701   A   G   SNP A   A   A   A/G A   A   A/G A   A   A   missense_variant    MODERATE    MISSENSE    Aca/Gca p.Thr6162Ala/c.18484A>G 6757    CDS_1   protein_coding
    PP810610    19028   C   T   SNP C   C   C   C/T C   C   C   C   C   C   stop_gained HIGH    NONSENSE    Caa/Taa p.Gln6271*/c.18811C>T   6757    CDS_1   protein_coding
    PP810610    19289   G   T   SNP G   G   T   G   G   G/T G   G   G/T G   missense_variant    MODERATE    MISSENSE    Gtt/Ttt p.Val6358Phe/c.19072G>T 6757    CDS_1   protein_coding
    PP810610    19294   C   T   SNP C   C   C   C   C   C/T C/T C   C/T C   synonymous_variant  LOW SILENT  taC/taT p.Tyr6359Tyr/c.19077C>T 6757    CDS_1   protein_coding
    PP810610    21027   C   T   SNP C   C/T C   C/T C/T C   C/T T   C   C/T missense_variant    MODERATE    MISSENSE    aCt/aTt p.Thr178Ile/c.533C>T    1173    CDS_2   protein_coding
    PP810610    21183   T   G   SNP G   G   G   G   G   G   G   G   G   G   missense_variant    MODERATE    MISSENSE    tTt/tGt p.Phe230Cys/c.689T>G    1173    CDS_2   protein_coding
    PP810610    21633   T   C   SNP T   T/C T   T   T   T   T   T   T   T   missense_variant    MODERATE    MISSENSE    gTt/gCt p.Val380Ala/c.1139T>C   1173    CDS_2   protein_coding
    PP810610    22215   T   G   SNP T   T   T   T/G T   T   T/G T   T   T   missense_variant    MODERATE    MISSENSE    gTt/gGt p.Val574Gly/c.1721T>G   1173    CDS_2   protein_coding
    PP810610    22487   A   G   SNP A   A   A   A   A   A/G A   A   A/G A   missense_variant    MODERATE    MISSENSE    Agt/Ggt p.Ser665Gly/c.1993A>G   1173    CDS_2   protein_coding
    PP810610    22630   C   T   SNP C   C   C   C   C   C   C   C   C   C/T synonymous_variant  LOW SILENT  taC/taT p.Tyr712Tyr/c.2136C>T   1173    CDS_2   protein_coding
    PP810610    22636   T   G   SNP G   G   G   G   G   G   G   G   G   G   missense_variant    MODERATE    MISSENSE    aaT/aaG p.Asn714Lys/c.2142T>G   1173    CDS_2   protein_coding
    PP810610    22763   G   T   SNP G   G   G   G   G   G   G   G   G/T G   missense_variant    MODERATE    MISSENSE    Gct/Tct p.Ala757Ser/c.2269G>T   1173    CDS_2   protein_coding
    PP810610    22788   T   C   SNP T   T   T   T   T   T/C T   T/C T/C T   missense_variant    MODERATE    MISSENSE    gTt/gCt p.Val765Ala/c.2294T>C   1173    CDS_2   protein_coding
    PP810610    23022   T   C   SNP C   C   C   C   C   C   C   C   C   C   missense_variant    MODERATE    MISSENSE    tTa/tCa p.Leu843Ser/c.2528T>C   1173    CDS_2   protein_coding
    PP810610    23435   C   T   SNP C   C   T   C/T C   C/T C/T C   C/T C   missense_variant    MODERATE    MISSENSE    Ctt/Ttt p.Leu981Phe/c.2941C>T   1173    CDS_2   protein_coding
    PP810610    24781   C   T,G SNP T   T   T   T   T   T   T   T   T   T/G missense_variant    MODERATE    MISSENSE    aCt/aGt p.Thr36Ser/c.107C>G 77  CDS_5   protein_coding
    PP810610    24971   A   G   SNP A   A   A   A   A   A   A   A   A/G A   missense_variant    MODERATE    MISSENSE    Aat/Gat p.Asn18Asp/c.52A>G  225 CDS_6   protein_coding
    PP810610    25025   C   T   SNP C   C/T C   C   C/T C   C   C/T C   C/T missense_variant    MODERATE    MISSENSE    Cac/Tac p.His36Tyr/c.106C>T 225 CDS_6   protein_coding
    PP810610    25163   C   T   SNP T   T   T   T   T   T   T   T   T   T   missense_variant    MODERATE    MISSENSE    Ctt/Ttt p.Leu82Phe/c.244C>T 225 CDS_6   protein_coding
    PP810610    25264   C   T   SNP T   T   T   T   T   T   T   T   T   T   synonymous_variant  LOW SILENT  gtC/gtT p.Val115Val/c.345C>T    225 CDS_6   protein_coding
    PP810610    25592   T   C   SNP T   T/C T   T   T/C T   T   T/C T   T/C missense_variant    MODERATE    MISSENSE    Ttc/Ctc p.Phe225Leu/c.673T>C    225 CDS_6   protein_coding
    PP810610    26104   C   T   SNP C   C   C   C   C   C   C   C   C   C/T missense_variant    MODERATE    MISSENSE    cCt/cTt p.Pro165Leu/c.494C>T    389 CDS_7   protein_coding
    PP810610    26838   G   T   SNP T   T   T   T   T   T   T   T   T   T                               
   
    PP810610    24731   TGTGGTGCTTATA   T   DEL TGTGGTGCTTATA   TGTGGTGCTTATA   TGTGGTGCTTATA   TGTGGTGCTTATA   TGTGGTGCTTATA   TGTGGTGCTTATA   TGTGGTGCTTATA   TGTGGTGCTTATA   T   TGTGGTGCTTATA   conservative_inframe_deletion           c.61_72delGTGCTTATAGTG  p.Val21_Val24del            

6. Calling intra-host variants using viral-ngs

    # #Install Gap2Seq in the docker-env --> generated the new docker-env viral-ngs-fixed:la
    # bin/assembly.py gapfill_gap2seq tmp/02_assembly/hCoV229E_Rluc.assembly2-scaffolded.fasta data/01_per_sample/hCoV229E_Rluc.cleaned.bam tmp/02_assembly/# hCoV229E_Rluc.assembly2-gapfilled.fasta --memLimitGb 12 --maskErrors --randomSeed 0
    # ----> go to the script tools/gap2seq.py, install the required tool (for example gap2seq) and adapt the correct version.
    # conda install -y -c bioconda gap2seq
    # root@f47daf7c44ee:/work# Gap2Seq -h
    # #>Gap2Seq 3.1
    # vim /home/jhuang/Tools/viral-ngs_docker/bin/tools/gap2seq.py
    # #Adapt the TOOL_NAME and TOOL_VERSION in the script
    #
    # #Save the docker-env with newly installed Gap2Seq
    # exit
    # docker ps -a
    # docker commit f47daf7c44ee viral-ngs-fixed:la
   
    #调用新的 docker-env having Gap2Seq
    docker run -it -v /mnt/md1/DATA_D/Data_Pietschmann_229ECoronavirus_Mutations_2026/viralngs:/work -v /home/jhuang/Tools/viral-ngs_docker:/home/jhuang/Tools/viral-ngs_docker -v /home/jhuang/REFs:/home/jhuang/REFs -v /home/jhuang/Tools/GenomeAnalysisTK-3.6:/home/jhuang/Tools/GenomeAnalysisTK-3.6 -v /home/jhuang/Tools/novocraft_v3:/home/jhuang/Tools/novocraft_v3 -v /usr/local/bin/gatk:/usr/local/bin/gatk   viral-ngs-fixed:la bash
    cd /work
    conda activate viral-ngs-env
    snakemake --directory /work --printshellcmds --cores 80
   
    # The complete running commands for the complete data in 2026 as follows:
   
    #-1- Run several times of docker viral-ngs-fixed:la so that all ${sample}.assembly2-scaffolded.fasta generated by running each time only a isolate (one record in samples-assembly.txt and empty in samples-runs.txt)
    docker run ...
    cd /work
    conda activate viral-ngs-env
    snakemake --directory /work --printshellcmds --cores 80
    # --> Note that tmp/02_assembly/${sample}.assembly2-scaffolded.fasta and tmp/02_assembly/${sample}.assembly2-gapfilled.fasta were generated!
   
    #-2- Then run the following commands: tmp/02_assembly/${sample}.assembly2-gapfilled.fasta --> tmp/02_assembly/${sample}.assembly3-modify.fasta
    for sample in DMSO_p10 K22_p10 X7523_p10    DMSO_p16 K22_p16 X7523_p16    DMSO_p26 K22_p26 X7523_p26; do
            #MANUALLY running the following commands!
            bin/assembly.py impute_from_reference tmp/02_assembly/${sample}.assembly2-gapfilled.fasta tmp/02_assembly/${sample}.assembly2-scaffold_ref.fasta tmp/02_assembly/${sample}.assembly3-modify.fasta --newName ${sample} --replaceLength 55 --minLengthFraction 0.05 --minUnambig 0.05 --index
    done
   
    #-3- Run docker for all isolates (full in amples-assembly.txt and samples-runs.txt).
    docker run ...
    cd /work
    conda activate viral-ngs-env
    snakemake --directory /work --printshellcmds --cores 80

7. Generate variant_annot.xls and coverages.xls

    sudo chown -R jhuang:jhuang data
    # -- generate isnvs_annot_complete__.txt, isnvs_annot_0.05.txt from ~/DATA/Data_Pietschmann_RSV_Probe3/data/04_intrahost
    cp isnvs.annot.txt isnvs.annot_complete.txt
    ~/Tools/csv2xls-0.4/csv_to_xls.py isnvs.annot_complete.txt -d$'\t' -o isnvs.annot_complete.xls
    #delete the columns patient, time, Hw and Hs and the header in the xls and save as txt file.
   
    awk '{printf "%.3f\n", $5}' isnvs.annot_complete.csv > f5
    cut -f1-4 isnvs.annot_complete.csv > f1_4
    cut -f6- isnvs.annot_complete.csv > f6_
    paste f1_4 f5 > f1_5
    paste f1_5 f6_ > isnvs_annot_complete_.txt
    #correct f5 in header of isnvs_annot_complete_.txt to iSNV_freq
    #Add header: chr    pos sample  alleles iSNV_freq   eff_type    eff_codon_dna   eff_aa  eff_aa_pos  eff_prot_len    eff_gene    eff_protein
    ~/Tools/csv2xls-0.4/csv_to_xls.py isnvs_annot_complete_.txt -d$'\t' -o variant_annot.xls
   
    #MANUALLY generate variant_annot_0.01.csv variant_annot_0.05.csv
    awk ' $5 >= 0.05 ' isnvs_annot_complete_.txt > 0.05.csv
    cut -f2 0.05.csv | uniq > ids_0.05
   
    awk ' $5 >= 0.02 ' isnvs_annot_complete_.txt > 0.02.csv
    cut -f2 0.02.csv | uniq > ids_0.02
   
    awk ' $5 >= 0.01 ' isnvs_annot_complete_.txt > 0.01.csv
    cut -f2 0.01.csv | uniq > ids_0.01
   
    #Replace '\n' with '\\t" isnvs_annot_complete_.txt >> isnvs_annot_0.05.txt\ngrep -P "PP810610\\t' in ids_0.05 and then deleting the 'pos' line
    #Replace '\n' with '\\t" isnvs_annot_complete_.txt >> isnvs_annot_0.01.txt\ngrep -P "PP810610\\t'  in ids_0.01 and then deleting the 'pos' line
    #Run ids_0.05 and ids_0.01
   
    cp ../../Outputs/Master_vcf/All_SNPs_indels_annotated.txt ../../Outputs/Master_vcf/All_SNPs_indels_annotated.txt hCoV229E_Rluc_variants
    #Manully adding the 3-way SNPs by getting original data from isnvs.annot.csv, for example,
    PP810610    8289    hCoV229E_Rluc   C,A,T   0.325, 0.439    missense_variant    8072C>A,8072C>T Ala2691Asp,Ala2691Val   2691    6758    Gene_217_20492  XBA84229.1
   
    # Delete the three records which already reported in intra-host results hCoV229E_Rluc_variants: they are 10871, 19289, 23435.
    PP810610       10871   C       T       SNP     C       C/T     T       C/T     C/T     T       C/T     missense_variant        MODERATE        MISSENSE        Ctt/Ttt p.Leu3552Phe/c.10654C>T 6757    CDS_1   protein_coding
    PP810610       19289   G       T       SNP     G       G       T       G       G       G/T     G       missense_variant        MODERATE        MISSENSE        Gtt/Ttt p.Val6358Phe/c.19072G>T 6757    CDS_1   protein_coding
    PP810610       23435   C       T       SNP     C       C       T       C/T     C       C/T     C/T     missense_variant        MODERATE        MISSENSE        Ctt/Ttt p.Leu981Phe/c.2941C>T   1173    CDS_2   protein_coding
   
    ~/Tools/csv2xls-0.4/csv_to_xls.py isnvs_annot_0.02.txt All_SNPs_indels_annotated.txt -d$'\t' -o variant_annot_2026.xls
    #Modify sheetname to variant_annot_0.05 and variant_annot_0.01 and add the header in Excel file.
    #Note in the complete list, Set 2024 is NOT a subset of Set 2025 because the element 26283 is in set 2024 but missing from set 2025.
   
    # -- calculate the coverage
    samtools depth ./data/02_align_to_self/hCoV229E_Rluc.mapped.bam > hCoV229E_Rluc_cov.txt
    samtools depth ./data/02_align_to_self/p10_DMSO.mapped.bam > p10_DMSO_cov.txt
    samtools depth ./data/02_align_to_self/p10_K22.mapped.bam > p10_K22_cov.txt
    samtools depth ./data/02_align_to_self/p10_K7523.mapped.bam > p10_K7523_cov.txt
    ~/Tools/csv2xls-0.4/csv_to_xls.py hCoV229E_Rluc_cov.txt p10_DMSO_cov.txt p10_K22_cov.txt p10_K7523_cov.txt -d$'\t' -o coverages.xls
    #draw coverage and see if they are continuous?
    samtools depth ./data/02_align_to_self/p16_DMSO.mapped.bam > p16_DMSO_cov.txt
    samtools depth ./data/02_align_to_self/p16_K22.mapped.bam > p16_K22_cov.txt
    samtools depth ./data/02_align_to_self/p16_X7523.mapped.bam > p16_K7523_cov.txt
    ~/Tools/csv2xls-0.4/csv_to_xls.py p16_DMSO_cov.txt p16_K22_cov.txt p16_K7523_cov.txt -d$'\t' -o coverages_p16.xls
   
            # Load required packages
            library(ggplot2)
            library(dplyr)
   
            # Read the coverage data
            cov_data <- read.table("p16_K7523_cov.txt", header = FALSE, sep = "\t",
                            col.names = c("Chromosome", "Position", "Coverage"))
   
            # Create full position range for the given chromosome
            full_range <- data.frame(Position = seq(min(cov_data$Position), max(cov_data$Position)))
   
            # Merge with actual coverage data and fill missing positions with 0
            cov_full <- full_range %>%
            left_join(cov_data[, c("Position", "Coverage")], by = "Position") %>%
            mutate(Coverage = ifelse(is.na(Coverage), 0, Coverage))
   
            # Save the plot to PNG
            png("p16_K7523_coverage_filled.png", width = 1200, height = 600)
   
            ggplot(cov_full, aes(x = Position, y = Coverage)) +
            geom_line(color = "steelblue", size = 0.3) +
            labs(title = "Coverage Plot for p16_K7523 (Missing = 0)",
            x = "Genomic Position",
            y = "Coverage Depth") +
            theme_minimal() +
            theme(
            plot.title = element_text(hjust = 0.5),
            axis.text = element_text(size = 10),
            axis.title = element_text(size = 12)
            )
   
            dev.off()

8. Comparing intra- and inter-host variants (40 positions are common between spandx and vphaser2)

    Please find attached the complete variant calling results for our 229E passaging experiment (2024–2026 datasets): variant_annot_2026__final.xls.
   
    • Sheet 1 (All_SNPs_Indels_annotated): Inter-host variants called by spandx. Shows consensus alleles at each variant position across all 10 samples relative to the PP810610 reference.
    • Sheet 2 (isnvs_annot): Intra-host variants called by vphaser2. Provides precise allele frequencies (iSNV_freq) per sample to quantify within-host diversity.
   
    Overlap:
   
    Green-highlighted rows indicate variants consistently detected by both pipelines.
    Sheet 2 is a subset of Sheet 1, focusing only on positions with intra-host heterogeneity. Fixed differences from the reference (where all 10 isolates share the same non-reference allele) remain in Sheet 1 (white rows). A few positions in Sheet 2 show iSNV_freq ≈ 1.0 (e.g., POS 15458, 22636). These reflect positions where vphaser2 detected minor variation in at least one sample, even if most samples show near-fixation.

9. (Optional) Consensus sequences of each and of all isolates

    cat PP810610.1.fa OZ035258.1.fa MZ712010.1.fa OK662398.1.fa OK625404.1.fa KF293664.1.fa NC_002645.1.fa > all.fa
    cp data/02_assembly/*.fasta ./
    for sample in hCoV229E_Rluc p10_DMSO p10_K22 p10_K7523; do \
    mv ${sample}.fasta ${sample}.fa
    cat all.fa ${sample}.fa >> all.fa
    done
   
    cat RSV_dedup.fa all.fa > RSV_all.fa
    mafft --clustalout --adjustdirection RSV_all.fa > RSV_all.aln
    snp-sites RSV_all.aln -o RSV_all_.aln