Seqanswers Leaderboard Ad

**HESmith** · 11-17-2011, 11:48 AM

Is there a reason not to use a custom sequencing primer?

**Simcom** · 11-17-2011, 12:19 PM

I am sequencing viral DNA/gDNA integration junctions, so I am using that 5 nucleotides of viral DNA as a type of 'verification', that indeed a read contains the junction between viral DNA and gDNA, essentially showing that the sequencing primer is not mis-hybridizing to a similar (non-viral) sequence elsewhere in the genome. We are using a custom sequencing primer, but we prefer that it not hybridize up the the very edge of the viral DNA for reason described above.

**GenoMax** · 11-17-2011, 12:29 PM

Can your core not run your samples by specifying a different lane (which is expected to have "normal" DNA) as the "control" lane for that run?

**HESmith** · 11-17-2011, 12:43 PM

Simcom: Judicious primer design coupled with the appropriate annealing temperature will virtually assure that the primer does not hybridize inappropriately.

Genomax: the designation of a normal complexity sample as the control lane does not solve the problem (sadly). While it allows the signal thresholds to be set appropriately, it doesn't address the problem of cluster resolution in the low complexity lanes.

**Simcom** · 11-17-2011, 12:50 PM

Originally posted by GenoMax View Post

Can your core not run your samples by specifying a different lane (which is expected to have "normal" DNA) as the "control" lane for that run?

I think you are misunderstanding the problem. The issue is, because the first 5nt of read #1 are going to be all identical among clusters, and the machine uses these 5nt to call clusters, the machine has a hard time identifying/differentiating between different clusters (especially close overlapping clusters). So the reason for the gDNA is to add diversity to the sequence, allowing clusters to be called. Hence the reason it needs to be included in the same lane as the sample.

**HESmith** · 11-17-2011, 12:53 PM

There's an alternative approach, assuming that you have not yet constructed the libraries. Design them so the junction is at the opposite end of the insert, and perform paired-end sequencing. Cluster calling is based only on the first five cycles of read one, so you'll avoid the low-complexity issue.

**Simcom** · 11-17-2011, 12:59 PM

Originally posted by HESmith View Post

Simcom: Judicious primer design coupled with the appropriate annealing temperature will virtually assure that the primer does not hybridize inappropriately.

I agree with you that hybridization is unlikely, but if it does happen it will be indistinguishable from an actual integration. Among other things, we are interested in mapping low-abundance integrations, so if we aren't able to get the verification sequence on every read, we will likely need to go in and verify a subset of integrations manually, which may not be possible if an integration is present in only one cell for example.

**Simcom** · 11-17-2011, 01:04 PM

Originally posted by HESmith View Post

There's an alternative approach, assuming that you have not yet constructed the libraries. Design them so the junction is at the opposite end of the insert, and perform paired-end sequencing. Cluster calling is based only on the first five cycles of read one, so you'll avoid the low-complexity issue.

Yep, exactly. Sadly my boss insisted on having a library that we can do single read OR paired end on (a money saving move potentially), so I had to design the junction on the first read side. And the samples are just about finished being prepped :/

**HESmith** · 11-17-2011, 01:05 PM

If, as you say, you can tolerate discarding 90-95% of the reads, then spiking in a gDNA library at that level will definitely solve your problem. After all, adapter dimers are often present at 5-10% in many libraries (the same % as your desired samples), and sequencing them is not a problem!

**Simcom** · 11-17-2011, 01:11 PM

Originally posted by HESmith View Post

If, as you say, you can tolerate discarding 90-95% of the reads, then spiking in a gDNA library at that level will definitely solve your problem. After all, adapter dimers are often present at 5-10% in many libraries (the same % as your desired samples), and sequencing them is not a problem!

Thanks, this gives me confidence. Just to be sure though: do the adapter-adapter ligation reads come back in the data, or does the machine throw them out and not include them in sequencing results? If you actually get the adapter-adapter reads from the machine, I should be golden.

**pmiguel** · 11-17-2011, 01:30 PM

We got it to work on our HiScanSQ -- which uses the same chemistry as the HiSeq, but only scans the top of the flowcell. Not an identical situation, but we had some SMART cDNAs that we sheared and ligated TruSeq adapters on. So about 1/2 of them had the same 50 nt of SMART primer at the beginning. We mixed them 1:1 with a genomic DNA library. Cluster registration went fine.

--
Phillip

**HESmith** · 11-17-2011, 01:32 PM

Yes, adapter reads are present.

Just remember that you'll also need to include the standard sequencing primer for the gDNA library (or construct the gDNA library with custom adapters to match your custom primer).

**Simcom** · 11-17-2011, 01:52 PM

Originally posted by HESmith View Post

Yes, adapter reads are present.

Just remember that you'll also need to include the standard sequencing primer for the gDNA library (or construct the gDNA library with custom adapters to match your custom primer).

Yep, I planned on including both primers. Thank you so much for your help, I really appreciate it.

**Simcom** · 11-17-2011, 02:00 PM

Originally posted by pmiguel View Post

We got it to work on our HiScanSQ -- which uses the same chemistry as the HiSeq, but only scans the top of the flowcell. Not an identical situation, but we had some SMART cDNAs that we sheared and ligated TruSeq adapters on. So about 1/2 of them had the same 50 nt of SMART primer at the beginning. We mixed them 1:1 with a genomic DNA library. Cluster registration went fine.

--
Phillip

OK, that is good to hear. I'm not sure why my core was having trouble spiking 1:1 gDNA.

Topics	Statistics	Last Post
AI Model Maps 3D Genome Structures in Minutes by seqadmin Started by seqadmin, 02-03-2025, 09:07 AM	0 responses 13 views 0 likes	Last Post by seqadmin 02-03-2025, 09:07 AM
Long-Read Sequencing Speeds Up Diagnosis of Rare Genetic Diseases by seqadmin Started by seqadmin, 01-31-2025, 08:31 AM	0 responses 26 views 0 likes	Last Post by seqadmin 01-31-2025, 08:31 AM
New Genome Analysis Tool Offers Scalable Phylogenomic Insights by seqadmin Started by seqadmin, 01-24-2025, 07:35 AM	0 responses 78 views 0 likes	Last Post by seqadmin 01-24-2025, 07:35 AM
How T Cells Protect the Gut from Infections by seqadmin Started by seqadmin, 01-23-2025, 09:43 AM	0 responses 47 views 0 likes	Last Post by seqadmin 01-23-2025, 09:43 AM

Seqanswers Leaderboard Ad

Announcement

Sequencing a Low diversity library on the HiSeq

Comment

Comment

Comment

Comment

Comment

Comment

Comment

Comment

Comment

Comment

Comment

Comment

Comment

Comment

Latest Articles

ad_right_rmr

News