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使用喷墨寡核苷酸合成仪制造的微阵列进行表达谱分析。

Expression profiling using microarrays fabricated by an ink-jet oligonucleotide synthesizer.

作者信息

Hughes T R, Mao M, Jones A R, Burchard J, Marton M J, Shannon K W, Lefkowitz S M, Ziman M, Schelter J M, Meyer M R, Kobayashi S, Davis C, Dai H, He Y D, Stephaniants S B, Cavet G, Walker W L, West A, Coffey E, Shoemaker D D, Stoughton R, Blanchard A P, Friend S H, Linsley P S

机构信息

Rosetta Inpharmatics, Inc., 12040 115th Avenue NE, Kirkland, WA 98034, USA.

出版信息

Nat Biotechnol. 2001 Apr;19(4):342-7. doi: 10.1038/86730.

Abstract

We describe a flexible system for gene expression profiling using arrays of tens of thousands of oligonucleotides synthesized in situ by an ink-jet printing method employing standard phosphoramidite chemistry. We have characterized the dependence of hybridization specificity and sensitivity on parameters including oligonucleotide length, hybridization stringency, sequence identity, sample abundance, and sample preparation method. We find that 60-mer oligonucleotides reliably detect transcript ratios at one copy per cell in complex biological samples, and that ink-jet arrays are compatible with several different sample amplification and labeling techniques. Furthermore, results using only a single carefully selected oligonucleotide per gene correlate closely with those obtained using complementary DNA (cDNA) arrays. Most of the genes for which measurements differ are members of gene families that can only be distinguished by oligonucleotides. Because different oligonucleotide sequences can be specified for each array, we anticipate that ink-jet oligonucleotide array technology will be useful in a wide variety of DNA microarray applications.

摘要

我们描述了一种灵活的基因表达谱分析系统,该系统使用通过采用标准亚磷酰胺化学的喷墨打印方法原位合成的数万个寡核苷酸阵列。我们已经表征了杂交特异性和灵敏度对包括寡核苷酸长度、杂交严谨性、序列同一性、样品丰度和样品制备方法等参数的依赖性。我们发现60聚体寡核苷酸能够可靠地检测复杂生物样品中每个细胞一个拷贝的转录本比率,并且喷墨阵列与几种不同的样品扩增和标记技术兼容。此外,每个基因仅使用一个精心挑选的寡核苷酸得到的结果与使用互补DNA(cDNA)阵列获得的结果密切相关。测量结果不同的大多数基因是只能通过寡核苷酸区分的基因家族成员。由于可以为每个阵列指定不同的寡核苷酸序列,我们预计喷墨寡核苷酸阵列技术将在各种DNA微阵列应用中发挥作用。

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