https://github.com/maragkakislab/samql

SQL-like query language for the SAM/BAM file format
https://github.com/maragkakislab/samql

bam bioinformatics go sam sequencing sql

Last synced: 26 days ago
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SQL-like query language for the SAM/BAM file format

• Host: GitHub
• URL: https://github.com/maragkakislab/samql
• Owner: maragkakislab
• License: mit
• Created: 2018-08-03T17:36:30.000Z (almost 6 years ago)
• Default Branch: master
• Last Pushed: 2023-09-20T16:58:03.000Z (9 months ago)
• Last Synced: 2024-02-09T08:38:43.554Z (4 months ago)
• Topics: bam, bioinformatics, go, sam, sequencing, sql
• Language: Go
• Homepage:
• Size: 65.4 KB
• Stars: 24
• Watchers: 5
• Forks: 5
• Open Issues: 0
• Metadata Files:
  • Readme: README.md
  • License: LICENSE

Lists

• awesome-bio-go - samql - like query language for the SAM/BAM file format. (Proteomics and Genomics Analysis)

README

        
# samql [![Go Report Card](https://goreportcard.com/badge/github.com/maragkakislab/samql)](https://goreportcard.com/report/github.com/maragkakislab/samql) [![GoDoc](https://godoc.org/github.com/maragkakislab/samql?status.svg)](https://godoc.org/github.com/maragkakislab/samql)

SQL-like query language for the SAM/BAM file format

## Install

Download the latest executable:

[Latest](https://github.com/maragkakislab/samql/releases/latest/).

Otherwise, to install the Go library and executable:

`go get github.com/maragkakislab/samql/...`

## Objective

To provide a command line utility and a clean API for filtering SAM/BAM files

using simple SQL-like commands. The samql command showcases the envisioned

functionality.

## Usage

```bash

Filters a SAM/BAM file using the SQL clause provided

samql 1.7

Usage: samql [--where WHERE] [--count] [--sam] [--parr PARR] [--obam] INPUT [INPUT ...]

Positional arguments:

  INPUT                  file (- for STDIN)

Options:

  --where WHERE          SQL clause to match records

  --count, -c            print only the count of matching records

  --sam, -S              interpret input as SAM, otherwise BAM

  --parr PARR, -p PARR   Number of cores for parallelization. Uses all available, if not provided.

  --obam, -b             Output BAM

  --help, -h             display this help and exit

  --version              display version and exit

```

## Examples

```bash

# Simple

samql --where "RNAME = chr1" test.bam    # Reference name is "chr1"

samql --where "QNAME = read1" test.bam   # Query name is "read1"

samql --where "POS > 100" test.bam       # Position (0-based) greater than 100

samql --where "REVERSE" test.bam         # Negative strand

samql --where "FLAG & 16 = 16" test.bam  # Ditto using flag arithmetics

# More than one files

samql --where "REVERSE" test1.bam test2.bam # Reads are returned in the order of the files

# Regex

samql --where "CIGAR =~ /^15M/" test.bam # Alignment starts with 15 matches

# More complex

samql --where "RNAME = chr1 OR QNAME = read1 AND POS > 100" test.bam

# Just counting

samql -c --where "RNAME = chr1" test.bam

# Very complex

# Uniquely mapped reads, with first pair on chr1 after

# position 1000000 and second pair on chr1 or chrX that

# start with 15 matches/mismatches, are shorter than 75 nts

# or begin with an ATG and are located on the reverse strand.

samql --where "(RNAME = 'chr1' AND POS > 1000000) AND \

               (RNEXT = 'chr1' OR RNEXT = 'chrX') AND \

               NH:i = 1 AND \

               CIGAR =~ /^15M/ AND \

               (LENGTH < 75 OR SEQ =~ /^ATG/) AND \

               PAIRED AND REVERSE"

```

## Keywords

```Go

QNAME         // QNAME corresponds to the SAM record query name.

FLAG          // FLAG corresponds to the SAM record alignment flag.

RNAME         // RNAME corresponds to the SAM record reference name

POS           // POS corresponds to the SAM record position (0-based).

MAPQ          // MAPQ corresponds to the SAM record mapping quality.

CIGAR         // CIGAR corresponds to the SAM record CIGAR string.

RNEXT         // RNEXT corresponds to the reference name of the mate read.

PNEXT         // PNEXT corresponds to the position of the mate read.

TLEN          // TLEN corresponds to SAM record template length.

SEQ           // SEQ corresponds to SAM record segment sequence.

QUAL          // QUAL corresponds to SAM record quality.

LENGTH        // LENGTH corresponds to the alignment length.

PAIRED        // PAIRED corresponds to SAM flag 0x1.

PROPERPAIR    // PROPERPAIR corresponds to SAM flag 0x2.

UNMAPPED      // UNMAPPED corresponds to SAM flag 0x4.

MATEUNMAPPED  // MATEUNMAPPED corresponds to SAM flag 0x8.

REVERSE       // REVERSE corresponds to SAM flag 0x10.

MATEREVERSE   // MATEREVERSE corresponds to SAM flag 0x20.

READ1         // READ1 corresponds to SAM flag 0x40.

READ2         // READ2 corresponds to SAM flag 0x80.

SECONDARY     // SECONDARY corresponds to SAM flag 0x100.

QCFAIL        // QCFAIL corresponds to SAM flag 0x200.

DUPLICATE     // DUPLICATE corresponds to SAM flag 0x400.

SUPPLEMENTARY // SUPPLEMENTARY corresponds to SAM flag 0x800.

END           // END corresponds to the alignment end.

```

## API example

```Go

// Open github.com/biogo/hts/sam reader

f := os.Open("test.sam")

sr, _ := sam.NewReader(f)

// Do the filtering

r := samql.NewReader(sr)

filter, _ := samql.Where("POS = 1")

r.Filters = append(r.Filters, filter)

for {

	rec, err := r.Read()

	if err != nil {

		if err == io.EOF {

			break

		}

		panic(err)

	}

	// Do sth with rec

}

```