Question

chip seq peaks are very long

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4.9 years ago

yiren ▴ 10

Hello ,every one, I have a question about peaks length.I get the peaks by macs2 for chipseq data(BAMPE file),but my peaks length is very long.they almost are bigger than 500 base. this is normal right?I will list some data from my peaks file below.Help me .Thank you very much!!

chr | star | end | length |  
chrR | 1888880 | 1897200 | 8320 | .
chr3 | 1030562 | 1036279 | 5717 | .
chr4 | 15450 | 21144 | 5694 | .
chr7 | 12389 | 17091 | 4702 | .
chr5 | 667728 | 671990 | 4262 | .
chr1 | 1475634 | 1479773 | 4139 | .
chr3 | 132973 | 136895 | 3922 | .
chr5 | 347409 | 351045 | 3636 | .
chr7 | 629367 | 632930 | 3563 | .
chr5 | 708703 | 712215 | 3512 | .
chr1 | 761428 | 764877 | 3449 | .
chr1 | 3146009 | 3149230 | 3221 | .
chr1 | 3105738 | 3108941 | 3203 | .
chr7 | 385703 | 388840 | 3137 | .
chr7 | 194748 | 197879 | 3131 | .
chr2 | 623495 | 626552 | 3057 | .
chr2 | 638941 | 641974 | 3033 | .
chrR | 1722466 | 1725316 | 2850 | .
chr2 | 1649317 | 1652141 | 2824 | .
chr1 | 1952043 | 1954826 | 2783 | .
chr2 | 804016 | 806797 | 2781 | .
chr4 | 1271810 | 1274566 | 2756 | .
chr1 | 661633 | 664373 | 2740 | .
chr6 | 86747 | 89481 | 2734 | .
chr1 | 2456965 | 2459657 | 2692 | .
chr2 | 522903 | 525579 | 2676 | .
chr1 | 3045426 | 3048054 | 2628 | .
chr1 | 190996 | 193613 | 2617 | .
chrR | 1586201 | 1588812 | 2611 | .
chr4 | 1041711 | 1044314 | 2603 | .
chr6 | 76212 | 78804 | 2592 | .
chr2 | 1746703 | 1749288 | 2585 | .
chr1 | 2432263 | 2434826 | 2563 | .
chr1 | 949260 | 951816 | 2556 | .
chr7 | 9592 | 12094 | 2502 | .
chr6 | 512863 | 515365 | 2502 | .
chr1 | 1509268 | 1511753 | 2485 | .
chrR | 988412 | 990843 | 2431 | .
chr7 | 439503 | 441929 | 2426 | .
chr2 | 180741 | 183107 | 2366 | .
chr1 | 1826541 | 1828905 | 2364 | .
chr4 | 1467570 | 1469922 | 2352 | .
chrR | 1762374 | 1764697 | 2323 | .
chr1 | 1526805 | 1529087 | 2282 | .

ChIP-Seq • 1.1k views

ADD COMMENT • link 4.9 years ago by yiren ▴ 10

score 1 · Answer 1 · 2020-01-15

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4.9 years ago

Devon Ryan 104k

Whether this is correct or not will depend on what you're IPing. How long do you expect it to be? Have you looked at some of the peaks and do they look reasonable? Use IGV.

ADD COMMENT • link 4.9 years ago by Devon Ryan 104k

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Most importantly, what did you ChIP? Broad histone mark, Pol-II?

ADD REPLY • link 4.9 years ago by ATpoint 85k

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It is Transcription factor.

ADD REPLY • link 4.9 years ago by yiren ▴ 10

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Can you show a browser track screenshot? It is unusual for TF peaks being that long. Can you also post a histogram or boxplot of the width across all peaks? Maybe you are picking up clusters of TFs in the example you show. How long were fragments after sonication? You can also check the insert size lengths in the paired-end bam file.

ADD REPLY • link 4.9 years ago by ATpoint 85k

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thank you for your reply.

ADD REPLY • link 4.9 years ago by yiren ▴ 10

score 1 · Answer 2 · 2020-01-15

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4.9 years ago

German.M.Demidov ★ 2.9k

May be your chip-seq mark is producing wide peaks? What is the difference between narrow peak, Broad peak and a gapped peak of a chip-seq experiment and is it okay to use all of these regions for downstream analysis Or you run MACS2 with the corresponding flag. I'd recommend to check https://bioinformatics.stackexchange.com/questions/4489/determine-if-chip-seq-peaks-are-broad-or-narrow and your mark (if it is a histone mark)