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鲍曼-伯克蛋白酶抑制剂基因编码区的一个四核苷酸碱基对缺失,阻止了其在小叶大豆PI440956种子中的积累。

A four-nucleotide base-pair deletion in the coding region of the Bowman-Birk protease inhibitor gene prevents its accumulation in the seeds of Glycine microphylla PI440956.

作者信息

Krishnan Hari B, Kim Won-Seok

机构信息

Plant Genetics Research Unit, USDA-ARS, University of Missouri, Columbia 65211, USA.

出版信息

Planta. 2003 Jul;217(3):523-7. doi: 10.1007/s00425-003-1050-3. Epub 2003 May 21.

Abstract

The Bowman-Birk protease inhibitor (BBI), an abundant soybean [ Glycine max (L.) Merr.] seed protein, is a major antinutritional factor. Nulls for the major soybean BBI have been reported in several of the wild perennial Glycine species including G. microphylla (Benth.) Tind PI440956. This perennial Glycine species does not accumulate the major BBI and the molecular basis for the absence of the major BBI in this plant introduction (PI) line is not known. We have cloned the BBI gene from G. microphylla PI440956, G. microphylla PI505188, and G. max cv. Jefferson and determined its nucleotide sequences. Analysis of the G. microphyllla PI505188 and G. max cv. Jefferson nucleotide sequences revealed a complete open-reading frame encoding the BBI. In contrast, the BBI coding region of G. microphylla PI440956 contained a frameshift mutation that resulted in the introduction of a stop codon at the amino terminal region of the protein. Reverse transcription-polymerase chain reaction analysis revealed that the BBI gene was expressed in developing seeds of G. microphylla PI505188 and G. max cv. Jefferson, but not in developing seeds of G. microphylla PI440956. In contrast, a BBI-related isoinhibitor gene was expressed at similar levels in all three Glycine species. Our results suggest that the frameshift mutation in the BBI coding region is responsible for the absence of BBI in the seeds of G. microphylla PI440956.

摘要

鲍曼-伯克蛋白酶抑制剂(BBI)是大豆[大豆(Glycine max (L.) Merr.)]种子中一种丰富的蛋白质,是主要的抗营养因子。在包括小叶大豆(G. microphylla (Benth.) Tind PI440956)在内的几种野生多年生大豆属物种中,已报道了主要大豆BBI的缺失突变体。这种多年生大豆属物种不积累主要的BBI,且该植物引进系(PI)中缺乏主要BBI的分子基础尚不清楚。我们已从小叶大豆PI440956、小叶大豆PI505188和大豆品种杰斐逊中克隆了BBI基因,并确定了其核苷酸序列。对小叶大豆PI505188和大豆品种杰斐逊的核苷酸序列分析揭示了一个编码BBI的完整开放阅读框。相比之下,小叶大豆PI440956的BBI编码区含有一个移码突变,导致在蛋白质的氨基末端区域引入了一个终止密码子。逆转录-聚合酶链反应分析表明,BBI基因在小叶大豆PI505188和大豆品种杰斐逊的发育种子中表达,但在小叶大豆PI440956的发育种子中不表达。相比之下,一个与BBI相关的同工抑制剂基因在所有三种大豆属物种中的表达水平相似。我们的结果表明,BBI编码区的移码突变是小叶大豆PI440956种子中缺乏BBI的原因。

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