Scaffolding of bacterial genome assemblies

0

Entering edit mode

3.4 years ago

Jelo • 0

Hi everyone,

I have bacterial genome sequenced by Illumina technology, the genome was de novo assembled by SPAdes assembler, I got 38 contigs. The contigs were reordered by Mauve using close reference genome. my question, is it correct to remove the headers between the contigs to produce only one scaffolds and do the annotation by PGAP tool? if I submit to NCBI in this case it will be accepted?

BTW, I tried to use gap filling tools, but that has no any effect.

I appreciate any help or advice in advance.

thank you

scaffolding genome annotation bacterial assembly • 1.1k views

ADD COMMENT • link updated 3.4 years ago by samuel.a.odonnell ▴ 580 • written 3.4 years ago by Jelo • 0

1

Entering edit mode

The contigs were reordered by Mauve using close reference genome. my question, is it correct to remove the headers between the contigs to produce only one scaffolds and do the annotation by PGAP tool?

No, you can't remove the headers and produce only one scaffold. The Mauve analysis only guess the order of the contigs based on a close reference genome. You must perform a PCR to confirm the exact order

ADD REPLY • link 3.4 years ago by andres.firrincieli 3.8k

0

Entering edit mode

I appreciate your reply

ADD REPLY • link 3.4 years ago by Jelo • 0

1

Entering edit mode

Generally scaffolding works somewhat like that except 'N's are placed in between the contigs to signify that they have been scaffolded together after assembly. This is only done within chromosomes too.

ADD REPLY • link 3.4 years ago by samuel.a.odonnell ▴ 580

Login before adding your answer.