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  • ChIP-Seq from Limited Starting Material of K562 Cells and Drosophila Neuroblasts Using Tagmentation Assisted Fragmentation Approach.

ChIP-Seq from Limited Starting Material of K562 Cells and Drosophila Neuroblasts Using Tagmentation Assisted Fragmentation Approach.

Bio-protocol (2021-03-04)
Junaid Akhtar, Piyush More, Steffen Albrecht
ABSTRACT

Chromatin immunoprecipitation is extensively used to investigate the epigenetic profile and transcription factor binding sites in the genome. However, when the starting material is limited, the conventional ChIP-Seq approach cannot be implemented. This protocol describes a method that can be used to generate the chromatin profiles from as low as 100 human or 1,000 Drosophila cells. The method employs tagmentation to fragment the chromatin with concomitant addition of sequencing adaptors. The method generates datasets with high signal to noise ratio and can be subjected to standard tools for ChIP-Seq analysis.

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Triton X-100, for molecular biology
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Formaldeide, for molecular biology, 36.5-38% in H2O
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Sodio cloruro, for molecular biology, DNase, RNase, and protease, none detected, ≥99% (titration)
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Glicina, BioUltra, for molecular biology, ≥99.0% (NT)
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Fenolo:cloroformio:alcool isoamilico 25:24:1, saturato con 10 mM di Tris, pH 8,0, 1 mM di EDTA, for molecular biology
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N,N-dimetilformammide, for molecular biology, ≥99%
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Ribonucleic acid, transfer from baker′s yeast (S. cerevisiae), Type X-SA, lyophilized powder
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Tris(idrossimetil)aminometano, ACS reagent, ≥99.8%
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