Literature DB >> 17406636

Global single-cell cDNA amplification to provide a template for representative high-density oligonucleotide microarray analysis.

Kazuki Kurimoto1, Yukihiro Yabuta, Yasuhide Ohinata, Mitinori Saitou.   

Abstract

We describe here a protocol for the representative amplification of global mRNAs from typical single mammalian cells to provide a template for high-density oligonucleotide microarray analysis. A single cell is lysed in a tube without purification and first-strand cDNAs are synthesized using a poly(dT)-tailed primer. Unreacted primer is specifically eliminated by exonuclease treatment and second strands are generated with a second poly(dT)-tailed primer after poly(dA) tailing of the first-strand cDNAs. The cDNAs are split into four tubes, which are independently directionally amplified by PCR, and then recombined. The amplified products (approximately 100 ng) show superior representation and reproducibility of original gene expression, especially for genes expressed in more than 20 copies per cell, compared with those obtained by a conventional PCR protocol, and can effectively be used for quantitative PCR and EST analyses. The cDNAs are then subjected to another PCR amplification with primers bearing the T7 promoter sequence. The resultant cDNA products are gel purified, amplified by one final cycle and used for isothermal linear amplification by T7 RNA polymerase to synthesize cRNAs for microarray hybridization. This protocol yields cDNA templates sufficient for more than 80 microarray hybridizations from a single cell, and can be completed in 5-6 days.

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Year:  2007        PMID: 17406636     DOI: 10.1038/nprot.2007.79

Source DB:  PubMed          Journal:  Nat Protoc        ISSN: 1750-2799            Impact factor:   13.491


  83 in total

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Authors:  Veronica Sanchez-Freire; Antje D Ebert; Tomer Kalisky; Stephen R Quake; Joseph C Wu
Journal:  Nat Protoc       Date:  2012-04-05       Impact factor: 13.491

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Review 3.  Single-cell analysis of the transcriptome and its application in the characterization of stem cells and early embryos.

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Journal:  Cell Mol Life Sci       Date:  2014-03-21       Impact factor: 9.261

Review 4.  Single-cell sequencing-based technologies will revolutionize whole-organism science.

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Journal:  Nat Rev Genet       Date:  2013-07-30       Impact factor: 53.242

5.  RNA-sequencing from single nuclei.

Authors:  Rashel V Grindberg; Joyclyn L Yee-Greenbaum; Michael J McConnell; Mark Novotny; Andy L O'Shaughnessy; Georgina M Lambert; Marcos J Araúzo-Bravo; Jun Lee; Max Fishman; Gillian E Robbins; Xiaoying Lin; Pratap Venepally; Jonathan H Badger; David W Galbraith; Fred H Gage; Roger S Lasken
Journal:  Proc Natl Acad Sci U S A       Date:  2013-11-18       Impact factor: 11.205

6.  Muscle IL1β Drives Ischemic Myalgia via ASIC3-Mediated Sensory Neuron Sensitization.

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7.  Complex genome-wide transcription dynamics orchestrated by Blimp1 for the specification of the germ cell lineage in mice.

Authors:  Kazuki Kurimoto; Yukihiro Yabuta; Yasuhide Ohinata; Mayo Shigeta; Kaori Yamanaka; Mitinori Saitou
Journal:  Genes Dev       Date:  2008-06-15       Impact factor: 11.361

8.  The cyclic gene Hes1 contributes to diverse differentiation responses of embryonic stem cells.

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Journal:  Genes Dev       Date:  2009-08-15       Impact factor: 11.361

9.  Incomplete inhibition of HIV infection results in more HIV infected lymph node cells by reducing cell death.

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Journal:  Elife       Date:  2018-03-20       Impact factor: 8.140

10.  Replication-coupled passive DNA demethylation for the erasure of genome imprints in mice.

Authors:  Saya Kagiwada; Kazuki Kurimoto; Takayuki Hirota; Masashi Yamaji; Mitinori Saitou
Journal:  EMBO J       Date:  2012-12-14       Impact factor: 11.598

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