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高粱(双色高粱)和大麦(大麦)中的淀粉分支酶:酶结构与基因表达的比较分析

Starch branching enzymes in sorghum (Sorghum bicolor) and barley (Hordeum vulgare): comparative analyses of enzyme structure and gene expression.

作者信息

Mutisya Joel, Sathish P, Sun Chuanxin, Andersson Lena, Ahlandsberg Staffan, Baguma Yona, Palmqvist Sara, Odhiambo Benjamin, Aman Per, Jansson Christer

机构信息

Department of Plant Biology, The Swedish University of Agricultural Sciences, P.O. Box 7080, SE-75007 Uppsala, Sweden.

出版信息

J Plant Physiol. 2003 Aug;160(8):921-30. doi: 10.1078/0176-1617-00960.

Abstract

A genomic clone for starch branching enzyme (SBE) IIb was isolated from a sorghum bacterial artificial chromosome (BAC) library. The promoter and 5' flanking sequence, the first four exons and introns as well as the last exon and the 3' untranslated region were sequenced. The tentative transcription start site of sorghum sbeIIb was mapped based on alignment with the maize sbeIIb gene. The exon-intron structure of the 5' portion of sorghum sbeIIb was similar to that of maize sbeIIb but differed from that of barley sbeIIb. Specifically, the intronic BbI element involved in the endosperm specific expression of barley sbeIIb was lacking in the sorghum gene. A cDNA clone for sorghum sbeIIb was reverse PCR amplified and found to encode an 803 amino acids long protein. The amino acid sequence of sorghum SBEIIb was compared to that of sorghum SBEI and corresponding enzymes in barley. The overall identity in amino acid sequence was 54% in the central portion of the enzymes. A major difference between the SBEII and SBEI isoforms was a 67 amino acids-long C-terminal extension in the SBEIs. The spatial and temporal expression patterns of sorghum sbeIIb was determined and compared with those of the sorghum gene for SBEI and the barley genes for SBEIIB and SBEI. All four genes exhibited a seed specific expression. However, while barley sbeIIb and sbeI transcripts were detected exclusively in the endosperm, the sorghum genes were expressed also in the embryo. The activity of sorghum sbeIIb and sbeI exhibited a late onset, with a peak of transcription at around 22 days after pollination. This is similar to the pattern of barley sbeI but different from that of barley sbeIIb, which showed a peak of transcription at 12 days after pollination.

摘要

从高粱细菌人工染色体(BAC)文库中分离出淀粉分支酶(SBE)IIb的基因组克隆。对启动子和5'侧翼序列、前四个外显子和内含子以及最后一个外显子和3'非翻译区进行了测序。基于与玉米sbeIIb基因的比对,确定了高粱sbeIIb的暂定转录起始位点。高粱sbeIIb 5'部分的外显子-内含子结构与玉米sbeIIb相似,但与大麦sbeIIb不同。具体而言,高粱基因中缺乏参与大麦sbeIIb胚乳特异性表达的内含子BbI元件。通过反向PCR扩增得到高粱sbeIIb的cDNA克隆,发现其编码一个803个氨基酸长的蛋白质。将高粱SBEIIb的氨基酸序列与高粱SBEI以及大麦中的相应酶进行了比较。酶中央部分的氨基酸序列总体一致性为54%。SBEII和SBEI同工型之间的一个主要差异是SBEI中有一个67个氨基酸长的C末端延伸。确定了高粱sbeIIb的时空表达模式,并与高粱SBEI基因以及大麦SBEIIB和SBEI基因的表达模式进行了比较。所有四个基因均表现出种子特异性表达。然而,虽然仅在胚乳中检测到大麦sbeIIb和sbeI转录本,但高粱基因在胚中也有表达。高粱sbeIIb和sbeI的活性出现较晚,授粉后约22天转录达到峰值。这与大麦sbeI的模式相似,但与大麦sbeIIb不同,后者在授粉后12天转录达到峰值。

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