Sequencing genomes from single cells by polymerase cloning

被引:290
作者
Zhang, Kun
Martiny, Adam C.
Reppas, Nikos B.
Barry, Kerrie W.
Malek, Joel
Chisholm, Sallie W.
Church, George M.
机构
[1] Harvard Univ, Sch Med, Dept Genet, Boston, MA 02115 USA
[2] MIT, Dept Civil & Environm Engn, Cambridge, MA 02139 USA
[3] US DOE, Joint Genome Inst, Walnut Creek, CA 94598 USA
[4] Agencourt Biosci, Beverly, MA 01915 USA
基金
美国国家科学基金会;
关键词
D O I
10.1038/nbt1214
中图分类号
Q81 [生物工程学(生物技术)]; Q93 [微生物学];
学科分类号
071005 ; 0836 ; 090102 ; 100705 ;
摘要
Genome sequencing currently requires DNA from pools of numerous nearly identical cells (clones), leaving the genome sequences of many difficult-to-culture microorganisms unattainable. We report a sequencing strategy that eliminates culturing of microorganisms by using real-time isothermal amplification to form polymerase clones (plones) from the DNA of single cells. Two Escherichia coli plones, analyzed by Affymetrix chip hybridization, demonstrate that plonal amplification is specific and the bias is randomly distributed. Whole-genome shotgun sequencing of Prochlorococcus MIT9312 plones showed 62% coverage of the genome from one plone at a sequencing depth of 3.5x, and 66% coverage from a second plone at a depth of 4.7x. Genomic regions not revealed in the initial round of sequencing are recovered by sequencing PCR amplicons derived from plonal DNA. The mutation rate in single-cell amplification is < 2 x 10(5), better than that of current genome sequencing standards. Polymerase cloning should provide a critical tool for systematic characterization of genome diversity in the biosphere.
引用
收藏
页码:680 / 686
页数:7
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