紫苏溶血磷脂酸酰基转移酶基因的克隆与功能分析

Cloning and functional characterization of a lysophosphatidic acid acyltransferase gene from Perilla frutescens

紫苏(Perillafrutescens)是一种重要食药同源油料作物,种子含油量高达46%-58%,其中α-亚麻酸(C18:3)含量占60%以上。溶血磷脂酸酰基转移酶(lysophosphatidicacid acyltransferase, LPAT)是植物种子三酰基甘油组装过程中的一类关键限速酶。本研究从紫苏发育种子中克隆了其编码基因(PfLPAT2),并利用qRT-PCR技术检测PfLPAT2基因在紫苏不同组织及不同发育时期种子的表达特性。构建PfLPAT2/GFP融合表达载体并通过农杆菌介导瞬时侵染本氏烟草叶片,检测PfLPAT2蛋白的亚细胞定位。构建大肠杆菌(Escherichia coli)表达载体、酵母表达载体和组成型植物过表达载体,分别转化大肠杆菌突变株SM2-1、酿酒酵母(Saccharomyces cerevisiae)野生型菌株INVSc1和普通烟草(Nicotiana tabacum),分析PfLPAT2蛋白的酶活性及生物学功能。结果表明,紫苏PfLPAT2基因ORF为1 155 bp,编码384个氨基酸。功能结构域预测显示PfLPAT2蛋白具有溶血磷脂酸酰基转移酶典型的保守区。PfLPAT2基因在紫苏根、茎、叶、花和开花后10、20、30、40 d的种子中均有表达,且在开花后20 d的种子中高表达。亚细胞定位结果显示PfLPAT2蛋白定位于细胞质。大肠杆菌功能互补测试表明,PfLPAT2可恢复SM2-1细胞膜脂生物合成,具有LPAT酶活性。与非转基因对照相比,转PfLPAT2基因酵母的总油脂含量显著提高,且脂肪酸各组分的含量发生改变,油酸(C18:1)含量增加明显,预示PfLPAT2对C18:1具有较高的底物偏好性。转基因烟草叶片总脂肪酸含量比对照组提高了约0.42倍,C18:1含量增加了约1倍。转基因株系总脂提高和脂肪酸组分的改变表明PfLPAT2异源表达可以促进宿主油脂合成和健康有益型脂肪酸(C18:1和C18:3)的积累。本研究为深入解析紫苏油脂特别是不饱和脂肪酸合成的分子调控机制和改良油料作物油脂品质提供理论依据和基因元件。

Perilla(Perilla frutescens L.)is an important edible-medicinal oil crop,with its seed containing 46%–58%oil.Of perilla seed oil,α-linolenic acid(C18:3)accounts for more than 60%.Lysophosphatidic acid acyltransferase(LPAT)is one of the key enzymes responsible for triacylglycerol assembly in plant seeds,controlling the metabolic flow from lysophosphatidic acid to phosphatidic acid.In this study,the LPAT2 gene from the developing seeds of perilla was cloned and designated as PfLPAT2.The expression profile of PfLPAT2 gene was examined in various tissues and different seed development stages of perilla(10,20,30,and 40 days after flowering,DAF)by quantitative real-time PCR(qRT-PCR).In order to detect the subcellular localization of PfLPAT2 protein,a fusion expression vector containing PfLPAT2 and GFP was constructed and transformed into Nicotiana benthamiana leaves by Agrobacterium-mediated infiltration.In order to explore the enzymatic activity and biological function of PfLPAT2 protein,an E.coli expression vector,a yeast expression vector and a constitutive plant overexpression vector were constructed and transformed into an E.coli mutant SM2-1,a wild-type Saccharomyces cerevisiae strain INVSc1,and a common tobacco(Nicotiana tabacum,variety:Sumsun NN,SNN),respectively.The results showed that the PfLPAT2 open reading frame(ORF)sequence was 1155 bp in length,encoding 384 amino acid residues.Functional structure domain prediction showed that PfLPAT2 protein has a typical conserved domain of lysophosphatidic acid acyltransferase.qRT-PCR analysis indicated that PfLPAT2 gene was expressed in all tissues tested,with the peak level in seed of 20 DAF of perilla.Subcellular localization prediction showed that PfLPAT2 protein is localized in cytoplasm.Functional complementation assay of PfLPAT2 in E.coli LPAAT mutant(SM2-1)showed that PfLPAT2 could restore the lipid biosynthesis of SM2-1 cell membrane and possess LPAT enzyme activity.The total oil content in the PfLPAT2 transgenic yeast was significantly increased,and the content of each fatty acid component changed compared with that of the non-transgenic control strain.Particularly,oleic acid(C18:1)in the transgenic yeast significantly increased,indicating that PfLPAT2 has a higher substrate preference for C18:1.Importantly,total fatty acid content in the transgenic tobacco leaves increased by about 0.42 times compared to that of the controls,with the C18:1 content doubled.The increased total oil content and the altered fatty acid composition in transgenic tobacco lines demonstrated that the heterologous expression of PfLPAT2could promote host oil biosynthesis and the accumulation of health-promoting fatty acids(C18:1 and C18:3).This study will provide a theoretical basis and genetic elements for in-depth analysis of the molecular regulation mechanism of perilla oil,especially the synthesis of unsaturated fatty acids,which is beneficial to the genetic improvement of oil quality of oil crops.