Dear all,

I have some sequencing results, however after trying to assembly them I got 3 different contigs. I know want to link those contigs so that I get 1 assembly (1 large plasmid).

Is it ok to just design primers at the exterior parts of the contigs in the hope I will have overlap between the contigs and this 1 large config rather than 3 small ones?

What I mean, schematically, is this:

contig 1

XXXXXX..............XXXXXX
<---- primer1 ......  primer 2 -->

Contig 2

YYYYY..................YYYYY
<---- primer 3 ......  primer 4 -->

Contig 3

ZZZZZZZZZZZZZ...........ZZZZZZZZZZZZ
<---- primer 5 ......  primer 6 -->

So I just design primers to sequence the endings further.

Or is there another trick?

Thanks in advance

You can certainly design primers to bridge gaps in your assembly if you are interested in closing gaps with Sanger sequencing, but you may be able to easily bridge gaps with your existing sequencing data.

You didn't provide us with any information on your sequencing data or how you assembled your reads, so we don't have any information on what you have done previously and how you might be able to use your existing reads (hopefully paired end reads) to provide information on how these assembly gaps may be bridged. It would also be helpful if you provided some information on where your sequences come from (organism) as existing knowledge about sequence diversity can help here also.

There are numerous tools to do this, but I would recommend certains tools over others based on the type of sequencing data you have, the length of gaps to be bridge (figure out from paired end reads), and the organism you are studying.

Can you provide us some more information by amending your original question?

All you have is PCR products which are Sanger sequenced, correct? People rarely assembly Sanger products anymore, but you can try software that should work well (Phrap, CAP3, etc...)