a modified protocol for bisulfite genomic sequencing of difficult samples修改后的协议样本亚硫酸氢基因组测序的困难.pdfVIP
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a modified protocol for bisulfite genomic sequencing of difficult samples修改后的协议样本亚硫酸氢基因组测序的困难
A Modified Protocol for Bisulfite Genomic Sequencing
of Difficult Samples
Jane J. Pappas, André Toulouse, and W. E. C. Bradley
Abstract
The bisulfite genomic sequencing protocol is a widely used method for analyzing DNA methylation. It relies
on the deamination of unmethylated cytosine residues to uracil; however, its high rates of DNA degradation
and incomplete cytosine to uracil conversion often lead to failed experiments, uninformative results, and false
positives. Here, we report the addition of a single-step multiple restriction enzyme digestion (MRED)
designed to differentially digest polymerase chain reaction products amplified from unconverted DNA while
leaving those of converted DNA intact. We show that for our model system, RARB2 P2 promoter, use of
MRED increased informative sequencings ninefold, and MRED did not alter the clonal representation in
one fully methylated cell line, H-596, treated or not with 5-azadeoxycytidine, a methylation inhibitor.
We believe that this method may easily be adapted for analyzing other genes and provide guidelines for
selecting the most appropriate MRED restriction enzymes.
Key words: bisulfite genomic sequencing, multiple restriction enzyme digestion, methylation.
1. Introduction
The bisulfite genomic sequencing (BGS) protocol ( 1, 2) is a
method of choice for analyzing DNA methylation at the nucleotide
level. Sodium bisulfite is used to convert unmethylated cytosine
residues to uracil residues in single-stranded DNA. In particular, bi-
sulfite conversion consists of three sequential chemical reactions:
sulfonation of cytosine to cytosine-6-sulfonate, deamination to
uracil-6-sulfonate, and desulfonation to uracil. However, since 5-
methylcy
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