Optimization of experimental design parameters for high-throughput chromatin immunoprecipitation studies.

Optimization of experimental design parameters for high-throughput chromatin immunoprecipitation studies.

Nucleic acids research (2008-10-23)

Romina Ponzielli, Paul C Boutros, Sigal Katz, Angelina Stojanova, Adam P Hanley, Fereshteh Khosravi, Christina Bros, Igor Jurisica, Linda Z Penn

PMID18940864

ABSTRACT

High-throughput, microarray-based chromatin immunoprecipitation (ChIP-chip) technology allows in vivo elucidation of transcriptional networks. However this complex is not yet readily accessible, in part because its many parameters have not been systematically evaluated and optimized. We address this gap by systematically assessing experimental-design parameters including antibody purity, dye-bias, array-batch, inter-day hybridization bias, amplification method and choice of hybridization control. The combined performance of these optimized parameters shows a 90% validation rate in ChIP-chip analysis of Myc genomic binding in HL60 cells using two different microarray platforms. Increased sensitivity and decreased noise in ChIP-chip assays will enable wider use of this methodology to accurately and affordably elucidate transcriptional networks.

MATERIALI

N° Catalogo

Marchio

Descrizione del prodotto

WGA2

Sigma-Aldrich

Kit completo di amplificazione dell′intero genoma (WGA) GenomePlex^®, Optimized kit with enzyme for amplifying a variety of DNA including FFPE tissue

R5500

Sigma-Aldrich

Ribonucleasi A, Type XII-A, ≥90% (SDS-PAGE), 75-125 Kunitz units/mg protein

D8661

Sigma-Aldrich

Deoxyribonucleic acid solution from calf thymus, For hybridization

WGA3

Sigma-Aldrich

GenomePlex^® WGA Reamplification Kit, Reamplification of WGA product with minimal bias