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在波士頓大學(xué),Pippin 使ChIP-seq Prep更加快速

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染色質(zhì)免疫共沉淀技術(shù)(Chromatin Immunoprecipitation,ChIP)也稱結(jié)合位點(diǎn)分析法,是研究體內(nèi)蛋白質(zhì)與DNA相互作用的有力工具,通常用于轉(zhuǎn)錄因子結(jié)合位點(diǎn)或組蛋白特異性修飾位點(diǎn)的研究。將ChIP與第二代測(cè)序技術(shù)相結(jié)合的ChIP-Seq技術(shù),能夠高效地在全基因組范圍內(nèi)檢測(cè)與組蛋白、轉(zhuǎn)錄因子等互作的DNA區(qū)段。
ChIP-Seq的原理是:首先通過染色質(zhì)免疫共沉淀技術(shù)(ChIP)特異性地富集目的蛋白結(jié)合的DNA片段,并對(duì)其進(jìn)行純化與文庫構(gòu)建;然后對(duì)富集得到的DNA片段進(jìn)行高通量測(cè)序。研究人員通過將獲得的數(shù)百萬條序列標(biāo)簽精確定位到基因組上,從而獲得全基因組范圍內(nèi)與組蛋白、轉(zhuǎn)錄因子等互作的DNA區(qū)段信息。
 

   At Boston University, the Galagan lab is trying to get a complete picture of Mycobacterium tuberculosis — in particular, how the organism’s regulatory network functions. By methodically performing ChIP-seq on each transcription factor in the microbe, the scientists are using sequence data to determine which other transcription factors and genomic regions are expressed as a result. The ultimate goal: a comprehensive view of the complex interactions among these transcription factors across the whole TB genome.

The scientist behind the lab’s library prep is Chris Mawhinney, who says that using Pippin Prep for size selection in the ChIP workflow saves her time and eliminates the possibility of sample cross-contamination. Mawhinney performs size selection after adapter ligation and purification as she preps libraries for sequencing on the Illumina GAIIx. “If you have too broad a range of sizes, the sequencer software has issues locating the clusters,” she says. “And adapter-dimers will anneal to your flow cell and eat up your reads, wasting capacity.”

Mawhinney uses Pippin to select for 250 base pairs, which allows her to remove the low molecular weight content as well as larger fragments. “With Pippin Prep, you can get it down to a really nice, narrow size,” she says, noting that the tool is easy to set up and run.

In addition to the time savings of using an automated solution instead of a manual gel, Mawhinney says Pippin speeds up the sample prep routine because there’s no cleanup needed. “The great thing about Pippin is that you can go right from size selection to PCR; there’s no middle cleanup step, so it’s very convenient,” she adds. “That’s a huge plus and it saves a lot of time.”

Preventing contamination is also critical in a lab where samples are often used up completely during sequencing. Mawhinney treats each sample as precious, so she can’t afford to lose anything to contamination or to poor sizing. On Pippin, she says, “the channels are all separate, so that gets rid of the possibility of contamination.”

For more on the Galagan lab’s interrogation of transcription factors in TB, check out their recent Nature paper.

 

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