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基于玉米表达序列标签频率分析和微阵列杂交的RNA表达谱比较

Comparison of RNA expression profiles based on maize expressed sequence tag frequency analysis and micro-array hybridization.

作者信息

Fernandes John, Brendel Volker, Gai Xiaowu, Lal Shailesh, Chandler Vicki L, Elumalai Rangasamy P, Galbraith David W, Pierson Elizabeth A, Walbot Virginia

机构信息

Department of Biological Sciences, Stanford University, Stanford, California 94305-5020, USA.

出版信息

Plant Physiol. 2002 Mar;128(3):896-910. doi: 10.1104/pp.010681.

Abstract

Assembly of 73,000 expressed sequence tags (ESTs) representing multiple organs and developmental stages of maize (Zea mays) identified approximately 22,000 tentative unique genes (TUGs) at the criterion of 95% identity. Based on sequence similarity, overlap between any two of nine libraries with more than 3,000 ESTs ranged from 4% to 20% of the constituent TUGs. The most abundant ESTs were recovered from only one or a minority of the libraries, and only 26 EST contigs had members from all nine EST sets (presumably representing ubiquitously expressed genes). For several examples, ESTs for different members of gene families were detected in distinct organs. To study this further, two types of micro-array slides were fabricated, one containing 5,534 ESTs from 10- to 14-d-old endosperm, and the other 4,844 ESTs from immature ear, estimated to represent about 2,800 and 2,500 unique genes, respectively. Each array type was hybridized with fluorescent cDNA targets prepared from endosperm and immature ear poly(A(+)) RNA. Although the 10- to 14-d-old postpollination endosperm TUGs showed only 12% overlap with immature ear TUGs, endosperm target hybridized with 94% of the ear TUGs, and ear target hybridized with 57% of the endosperm TUGs. Incomplete EST sampling of low-abundance transcripts contributes to an underestimate of shared gene expression profiles. Reassembly of ESTs at the criterion of 90% identity suggests how cross hybridization among gene family members can overestimate the overlap in genes expressed in micro-array hybridization experiments.

摘要

对代表玉米(Zea mays)多个器官和发育阶段的73000个表达序列标签(EST)进行组装,以95%的同一性标准鉴定出约22000个暂定独特基因(TUG)。基于序列相似性,九个EST文库中任意两个文库(每个文库有超过3000个EST)之间的重叠范围为组成TUG的4%至20%。最丰富的EST仅从一个或少数几个文库中回收,只有26个EST重叠群有来自所有九个EST组的成员(可能代表普遍表达的基因)。例如,在不同器官中检测到基因家族不同成员的EST。为了进一步研究,制作了两种类型的微阵列玻片,一种包含来自授粉后10至14天胚乳的5534个EST,另一种包含来自未成熟穗的4844个EST,估计分别代表约2800个和2500个独特基因。每种阵列类型都与从胚乳和未成熟穗的聚腺苷酸(+)RNA制备的荧光cDNA靶标杂交。尽管授粉后10至14天的胚乳TUG与未成熟穗TUG仅显示12%的重叠,但胚乳靶标与94%的穗TUG杂交,穗靶标与57%的胚乳TUG杂交。低丰度转录本的EST采样不完整导致对共享基因表达谱的低估。以90%的同一性标准对EST进行重新组装表明,基因家族成员之间的交叉杂交如何在微阵列杂交实验中高估表达基因的重叠。

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