Kajikawa Masataka, Yamaoka Shohei, Yamato Katsuyuki T, Kanamaru Hiroyuki, Sakuradani Eiji, Shimizu Sakayu, Fukuzawa Hideya, Ohyama Kanji
Laboratory of Plant Molecular Biology, Division of Integrated Life Science, Graduate School of Biostudies, Kyoto University, Kyoto 606-8502, Japan.
Biosci Biotechnol Biochem. 2003 Mar;67(3):605-12. doi: 10.1271/bbb.67.605.
We have isolated a beta-ketoacyl CoA synthase (KCS) gene, MpFAE2, from a liverwort, Marchantia polymorpha, and identified its substrate specificity using the technique of dsRNA-mediated gene silencing and overexpression. KCS catalyzes an essential reaction in the fatty acid elongation process, i.e., condensation of malonyl-CoA with acyl-CoA. By introducing a construct with a hairpin structure containing a partial MpFAE2 gene, the level of the MpFAE2 gene expression was suppressed constitutively. The transgenic plants showed a specific accumulation of fatty acid 18:0. In contrast, in transgenic M. polymorpha plants overexpressing the MpFAE2 gene, fatty acid 22:0 is accumulated. These results indicate that the MpFAE2 gene product catalyzes the elongation steps of 18:0 to 20:0 and possibly also of 20:0 to 22:0.
我们从苔类植物多歧藻(Marchantia polymorpha)中分离出了一个β-酮脂酰辅酶A合酶(KCS)基因MpFAE2,并使用双链RNA介导的基因沉默和过表达技术确定了其底物特异性。KCS催化脂肪酸延长过程中的一个关键反应,即丙二酸单酰辅酶A与酰基辅酶A的缩合反应。通过导入一个含有部分MpFAE2基因的发夹结构构建体,MpFAE2基因的表达水平被持续抑制。转基因植物表现出脂肪酸18:0的特异性积累。相反,在过表达MpFAE2基因的转基因多歧藻植物中,脂肪酸22:0得以积累。这些结果表明,MpFAE2基因产物催化了从18:0到20:0以及可能从20:0到22:0的延长步骤。
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