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**ychang** · 03-05-2013, 04:09 PM

we have succeed make 4-7kb mate-pair lib with Nextera kit, and will try 10kb this week.

**aammar** · 03-27-2013, 01:00 PM

Hi ychang,

I just started using the Nextera MP kit. How did you manage that short of kb insert? I get them on the larger side. I ideally want 3-4 kb insert size. Suggestions? Thank you in advance!

**jjcooper** · 05-09-2013, 06:53 PM

Hi ychang,
Did you have any luck with the 10 kb prep?
Hi aammar,
What size do your insert sizes usually end up? are you using the gel-plus protocol?
Thanks

**MLog** · 05-10-2013, 05:00 AM

Hi ychang (and everyone who has experience with Nextera MP, too),
did you already sequenced and mapped these libraries? I wonder how many reads mapped with expected insert size?
I tried Nextera MP for the first time, but the results are a bit disappointing - only ~ 40% of reads map in correct orientation and with expected insert size. The rest 60% seem to be short fragments that yield standard paired-end reads.

Attached Files

Fesc_3-4C_hist.png (9.6 KB, 69 views)

**Ama** · 05-15-2013, 03:38 PM

Hi

@MLog: I assume you removed the junction adapters of the nextera data before you did the mapping, can you please let me know what tools/approach you used for that? I been following the technical notes to trim the adapters off and to identify the reads orientation RF/FR, but the results I am seeing are very disappointing. So any help would be much appreciated.
Thanks

**jjcooper** · 05-15-2013, 04:30 PM

@MLog,
Did you do the gel-free or gel-plus protocol? How did your QCs with the Bioanalyzer look?

**syfo** · 05-16-2013, 04:10 AM

You might also need to reverse complement the reads before mapping them because some aligners expect the mates to be in a convergent orientation (head-to-head).

**sara_ahmed** · 05-16-2013, 06:13 AM

What is the circularization efficiency using the Nextera MP protocol? Is there a way to assess that in the protocol?

**hfaoro** · 08-02-2013, 07:49 AM

Hi,
About nextera MP protocol, does anyone knows if is it possible to use covaris microTUBE with fiber, instead of T6 tube, to shear the DNA after circularization step?

**BobS** · 08-06-2013, 03:14 PM

hfaoro , we used to use microTubes also.
Covaris Fragmentation for about 400bp fragments: For each 300ul + 9ul + 12ul reaction add 80 ul TE to bring volume up to near 400 ul microTube. Load 3 , 6 x 16 mm MicroTubes per sample 3 x 130ul = 390ul

Covaris E210 settings for ~400 bp fragments
5% Duty Cycle, 3 Intensity, 200 Cycles per burst, 110 sec. duration water cooled at 6 - 8 deg C. You probably will have to tweak your settings.

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