Bowtie 2 seems to be working fine (tested command '/home/shared/bowtie2-2.4.4-linux-x86_64/bowtie2 --version' [2.4.4])
Output format is BAM (default)
Alignments will be written out in BAM format. Samtools found here: '/usr/bin/samtools'
Reference genome folder provided is ../data/	(absolute path is '/home/shared/8TB_HDD_03/sr320/github/timeseries_molecular/E-Peve/data/)'
FastQ format assumed (by default)
Processing sequences up to read no. 10000 from the input file
Attention: using more than 4 cores per alignment thread has been reported to have diminishing returns. If possible try to limit -p to a value of 4
Each Bowtie 2 instance is going to be run with 8 threads. Please monitor performance closely and tune down if necessary!

Input files to be analysed (in current folder '/home/shared/8TB_HDD_03/sr320/github/timeseries_molecular/E-Peve/code'):
../data/03-Peve-bismark/POR-260-TP4_R1_001.fastp-trim.fq.gz
../data/03-Peve-bismark/POR-260-TP4_R2_001.fastp-trim.fq.gz
Library is assumed to be strand-specific (directional), alignments to strands complementary to the original top or bottom strands will be ignored (i.e. not performed!)
Output will be written into the directory: /home/shared/8TB_HDD_03/sr320/github/timeseries_molecular/E-Peve/output/03-Peve-bismark/
Setting parallelization to single-threaded (default)

Summary of all aligner options:	-q --score-min L,0,-0.6 -p 8 --reorder --ignore-quals --no-mixed --no-discordant --dovetail --maxins 500
Current working directory is: /home/shared/8TB_HDD_03/sr320/github/timeseries_molecular/E-Peve/code

Now reading in and storing sequence information of the genome specified in: /home/shared/8TB_HDD_03/sr320/github/timeseries_molecular/E-Peve/data/

Single-core mode: setting pid to 1

Paired-end alignments will be performed
=======================================

The provided filenames for paired-end alignments are ../data/03-Peve-bismark/POR-260-TP4_R1_001.fastp-trim.fq.gz and ../data/03-Peve-bismark/POR-260-TP4_R2_001.fastp-trim.fq.gz
Input files are in FastQ format
Processing reads up to sequence no. 10000 from ../data/03-Peve-bismark/POR-260-TP4_R1_001.fastp-trim.fq.gz
Writing a C -> T converted version of the input file POR-260-TP4_R1_001.fastp-trim.fq.gz to POR-260-TP4_R1_001.fastp-trim.fq.gz_C_to_T.fastq

Created C -> T converted version of the FastQ file POR-260-TP4_R1_001.fastp-trim.fq.gz (10001 sequences in total)


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Processing reads up to sequence no. 10000 from ../data/03-Peve-bismark/POR-260-TP4_R2_001.fastp-trim.fq.gz
Writing a G -> A converted version of the input file POR-260-TP4_R2_001.fastp-trim.fq.gz to POR-260-TP4_R2_001.fastp-trim.fq.gz_G_to_A.fastq

Created G -> A converted version of the FastQ file POR-260-TP4_R2_001.fastp-trim.fq.gz (10001 sequences in total)

Input files are POR-260-TP4_R1_001.fastp-trim.fq.gz_C_to_T.fastq and POR-260-TP4_R2_001.fastp-trim.fq.gz_G_to_A.fastq (FastQ)
Now running 2 instances of Bowtie 2 against the bisulfite genome of /home/shared/8TB_HDD_03/sr320/github/timeseries_molecular/E-Peve/data/ with the specified options: -q --score-min L,0,-0.6 -p 8 --reorder --ignore-quals --no-mixed --no-discordant --dovetail --maxins 500

Now starting a Bowtie 2 paired-end alignment for CTread1GAread2CTgenome (reading in sequences from POR-260-TP4_R1_001.fastp-trim.fq.gz_C_to_T.fastq and POR-260-TP4_R2_001.fastp-trim.fq.gz_G_to_A.fastq, with the options: -q --score-min L,0,-0.6 -p 8 --reorder --ignore-quals --no-mixed --no-discordant --dovetail --maxins 500 --norc))
Found first alignment:
LH00526:197:22KFKVLT4:3:1101:43638:1070_1:N:0:CTTGCTAG+GGAGATGA/1	77	*	0	0	*	*	0	0	GGGAAAATAATTTTAAGAAAATTTTATGATTAAGAAATTATTTTTATTAGGTATATTATAGATTATATAAATGTGGTTTTGTATTTAGTTTTGTAAGTGATTGTTTAATTTTTAATGGAGTAAATGAAATTAATT	IIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIII-IIIIIIIIII9IIII9IIIIII-IIIIII9IIIIIIIIIIIIIIIIIIIII	YT:Z:UP
LH00526:197:22KFKVLT4:3:1101:43638:1070_2:N:0:CTTGCTAG+GGAGATGA/2	141	*	0	0	*	*	0	0	TCAAATAATCTACACTCTACATAAACCATTCCTAATATTACTATTACTTTACTTAATACCTTAAAAATTAATTTCATTTACTCCATTAAAAATTAAACAATCACTTACAAAACTAAATACAAAACCACATTTATA	IIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIII-IIIIIIIIIIIIIIIIIIIIIIIIIII-IIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIII	YT:Z:UP
Now starting a Bowtie 2 paired-end alignment for CTread1GAread2GAgenome (reading in sequences from POR-260-TP4_R1_001.fastp-trim.fq.gz_C_to_T.fastq and POR-260-TP4_R2_001.fastp-trim.fq.gz_G_to_A.fastq, with the options: -q --score-min L,0,-0.6 -p 8 --reorder --ignore-quals --no-mixed --no-discordant --dovetail --maxins 500 --nofw))
Found first alignment:
LH00526:197:22KFKVLT4:3:1101:43638:1070_1:N:0:CTTGCTAG+GGAGATGA/1	83	Porites_evermani_scaffold_962_GA_converted	147248	42	135M	=	147183	-200	AATTAATTTCATTTACTCCATTAAAAATTAAACAATCACTTACAAAACTAAATACAAAACCACATTTATATAATCTATAATATACCTAATAAAAATAATTTCTTAATCATAAAATTTTCTTAAAATTATTTTCCC	IIIIIIIIIIIIIIIIIIIII9IIIIII-IIIIII9IIII9IIIIIIIIII-IIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIII	AS:i:0	XN:i:0	XM:i:0	XO:i:0	XG:i:0	NM:i:0	MD:Z:135	YS:i:0	YT:Z:CP
LH00526:197:22KFKVLT4:3:1101:43638:1070_2:N:0:CTTGCTAG+GGAGATGA/2	163	Porites_evermani_scaffold_962_GA_converted	147183	42	135M	=	147248	200	TCAAATAATCTACACTCTACATAAACCATTCCTAATATTACTATTACTTTACTTAATACCTTAAAAATTAATTTCATTTACTCCATTAAAAATTAAACAATCACTTACAAAACTAAATACAAAACCACATTTATA	IIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIII-IIIIIIIIIIIIIIIIIIIIIIIIIII-IIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIII	AS:i:0	XN:i:0	XM:i:0	XO:i:0	XG:i:0	NM:i:0	MD:Z:135	YS:i:0	YT:Z:CP

>>> Writing bisulfite mapping results to POR-260-TP4_R1_001.fastp-trim_bismark_bt2_pe.bam <<<


Reading in the sequence files ../data/03-Peve-bismark/POR-260-TP4_R1_001.fastp-trim.fq.gz and ../data/03-Peve-bismark/POR-260-TP4_R2_001.fastp-trim.fq.gz
Chromosomal sequence could not be extracted for	LH00526:197:22KFKVLT4:3:1101:46543:2681_1:N:0:CTTGCTAG+GGAGATGA	Porites_evermani_scaffold_7327	1
Chromosomal sequence could not be extracted for	LH00526:197:22KFKVLT4:3:1101:5354:5987_1:N:0:CTTGCTAG+GGAGATGA	Porites_evermani_scaffold_1477	124972
10000 reads; of these:
  10000 (100.00%) were paired; of these:
    5099 (50.99%) aligned concordantly 0 times
    2783 (27.83%) aligned concordantly exactly 1 time
    2118 (21.18%) aligned concordantly >1 times
49.01% overall alignment rate
10000 reads; of these:
  10000 (100.00%) were paired; of these:
    5056 (50.56%) aligned concordantly 0 times
    2812 (28.12%) aligned concordantly exactly 1 time
    2132 (21.32%) aligned concordantly >1 times
49.44% overall alignment rate
Processed 10000 sequences in total

Failed to close filehandle AMBIG_1: Bad file descriptor at /home/shared/Bismark-0.24.0/bismark line 2641, <IN2> line 40004.
Failed to close filehandle AMBIG_2: Bad file descriptor at /home/shared/Bismark-0.24.0/bismark line 2642, <IN2> line 40004.
Failed to close filehandle UNMAPPED_1: Bad file descriptor at /home/shared/Bismark-0.24.0/bismark line 2643, <IN2> line 40004.
Failed to close filehandle UNMAPPED_2: Bad file descriptor at /home/shared/Bismark-0.24.0/bismark line 2644, <IN2> line 40004.

Successfully deleted the temporary files POR-260-TP4_R1_001.fastp-trim.fq.gz_C_to_T.fastq and POR-260-TP4_R2_001.fastp-trim.fq.gz_G_to_A.fastq

Final Alignment report
======================
Sequence pairs analysed in total:	10000
Final Cytosine Methylation Report
=================================
Total number of C's analysed:	348613

Total methylated C's in CpG context:	4898
Total methylated C's in CHG context:	289
Total methylated C's in CHH context:	937
Total methylated C's in Unknown context:	7

Total unmethylated C's in CpG context:	49974
Total unmethylated C's in CHG context:	60634
Total unmethylated C's in CHH context:	231881
Total unmethylated C's in Unknown context:	374

C methylated in CpG context:	8.9%
C methylated in CHG context:	0.5%
C methylated in CHH context:	0.4%
C methylated in unknown context (CN or CHN):	1.8%


Bismark completed in 0d 0h 0m 16s

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Bismark run complete
====================


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