Question

illumina: Adapter Confusion

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5 hours ago

lingjun meng ▴ 20

When learning about NGS library construction,I have a problem:

Library is automatically denatured into single strands and further diluted onboard the instrument.

It feels like double strands are used as input,and we may get two reads representing the same fragment.

A typical library like this:

enter image description here

After pcr,it seems like:

enter image description here

So are both the black forward strand and the gray reverse strand sequenced? Will it cause any problem?

ILLUMINA ADAPTER • 102 views

ADD COMMENT • link updated 2 hours ago by GenoMax 149k • written 5 hours ago by lingjun meng ▴ 20

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Cant edit answer because of the great fire wall

ADD REPLY • link 4 hours ago by lingjun meng ▴ 20

score 0 · Answer 1 · 2025-03-13

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4 hours ago

lieven.sterck 15k

unless you are using a strand specific protocol (very common nowadays, perhaps even default now) , both strands will be sequenced.

In general this will not cause any problems for downstream analyses. This situation is usually 'resolved' by for instance the read mapping software. Most of the times reads mapping to the sense or anti-sense of a locus are simply "grouped" to get an end result (eg in gene expression analysis).

ADD COMMENT • link 4 hours ago by lieven.sterck 15k

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Even for regular libraries, aligners will report alignments (if they are on the bottom strand) using appropriate SAM flags.

ADD REPLY • link 2 hours ago by GenoMax 149k