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质体溶血磷脂酰酰基转移酶对拟南芥胚胎发育至关重要。

Plastid lysophosphatidyl acyltransferase is essential for embryo development in Arabidopsis.

作者信息

Kim Hyun Uk, Huang Anthony H C

机构信息

Center for Plant Cell Biology, Department of Botany and Plant Sciences, University of California, Riverside, California 92521, USA.

出版信息

Plant Physiol. 2004 Mar;134(3):1206-16. doi: 10.1104/pp.103.035832. Epub 2004 Feb 19.

Abstract

Lysophosphatidyl acyltransferase (LPAAT) is a pivotal enzyme controlling the metabolic flow of lysophosphatidic acid into different phosphatidic acids in diverse tissues. A search of the Arabidopsis genome database revealed five genes that could encode LPAAT-like proteins. We identified one of them, LPAAT1, to be the lone gene that encodes the plastid LPAAT. LPAAT1 could functionally complement a bacterial mutant that has defective LPAAT. Bacteria transformed with LPAAT1 produced LPAAT that had in vitro enzyme activity much higher on 16:0-coenzyme A than on 18:1-coenzyme A in the presence of 18:1-lysophosphatidic acid. LPAAT1 transcript was present in diverse organs, with the highest level in green leaves. A mutant having a T-DNA inserted into LPAAT1 was identified. The heterozygous mutant has no overt phenotype, and its leaf acyl composition is similar to that of the wild type. Selfing of a heterozygous mutant produced normal-sized and shrunken seeds in the Mendelian ratio of 3:1, and the shrunken seeds could not germinate. The shrunken seeds apparently were homozygous of the T-DNA-inserted LPAAT1, and development of the embryo within them was arrested at the heart-torpedo stage. This embryo lethality could be rescued by transformation of the heterozygous mutant with a 35S:LPAAT1 construct. The current findings of embryo death in the homozygous knockout mutant of the plastid LPAAT contrasts with earlier findings of a normal phenotype in the homozygous mutant deficient of the plastid glycerol-3-phosphate acyltransferase; both mutations block the synthesis of plastid phosphatidic acid. Reasons for the discrepancy between the contrasting phenotypes of the two mutants are discussed.

摘要

溶血磷脂酰酰基转移酶(LPAAT)是一种关键酶,可控制溶血磷脂酸在不同组织中向不同磷脂酸的代谢流。对拟南芥基因组数据库的搜索揭示了五个可能编码LPAAT样蛋白的基因。我们鉴定出其中一个基因LPAAT1是编码质体LPAAT的唯一基因。LPAAT1可以在功能上互补具有缺陷LPAAT的细菌突变体。用LPAAT1转化的细菌产生的LPAAT在18:1 - 溶血磷脂酸存在的情况下,对16:0 - 辅酶A的体外酶活性比对18:1 - 辅酶A的活性高得多。LPAAT1转录本存在于不同器官中,在绿叶中的水平最高。鉴定出一个T - DNA插入LPAAT1的突变体。杂合突变体没有明显的表型,其叶片酰基组成与野生型相似。杂合突变体自交产生正常大小和皱缩种子,比例符合孟德尔的3:1,皱缩种子不能发芽。皱缩种子显然是T - DNA插入的LPAAT1的纯合子,其中胚胎的发育在心形 - 鱼雷形阶段停滞。通过用35S:LPAAT1构建体转化杂合突变体可以挽救这种胚胎致死性。目前质体LPAAT纯合敲除突变体中胚胎死亡的发现与早期质体甘油 - 3 - 磷酸酰基转移酶缺陷的纯合突变体中正常表型的发现形成对比;这两种突变都阻断了质体磷脂酸的合成。讨论了这两种突变体对比表型之间差异的原因。

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