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番茄(Solanum lycopersicum)新型质外体转化酶抑制剂的分子克隆、表达与特性分析及其在纯化液泡转化酶中的应用

Molecular cloning, expression and characterization of a novel apoplastic invertase inhibitor from tomato (Solanum lycopersicum) and its use to purify a vacuolar invertase.

作者信息

Reca Ida Barbara, Brutus Alexandre, D'Avino Rossana, Villard Claude, Bellincampi Daniela, Giardina Thierry

机构信息

ISM2/BiosCiences UMR CNRS 6263, Université Aix Marseille III/CNRS, Ingénierie et Mécanismes d'Action des Glycosidases, Université Paul Cézanne, 13397 Marseille Cedex 20, France.

出版信息

Biochimie. 2008 Nov-Dec;90(11-12):1611-23. doi: 10.1016/j.biochi.2008.04.019. Epub 2008 Jun 5.

DOI:10.1016/j.biochi.2008.04.019
PMID:18573306
Abstract

Protein inhibitors are molecules secreted by many plants. In a functional genomics approach, an invertase inhibitor (SolyCIF) of Solanum lycopersicum was identified at the Solanaceae Cornell University data bank (www.sgn.cornell.edu). It was established that this inhibitor is expressed mainly in the leaves, flowers and green fruit of the plant and localized in the cell wall compartment. The SolyCIF cDNA was cloned by performing RT-PCR, fully sequenced and heterologously expressed in Pichia pastoris X-33. The purified recombinant protein obtained by performing ion-exchange chromatography and gel filtration was further biochemically characterized and used to perform affinity chromatography. The latter step made it possible to purify natural vacuolar invertase (TIV-1), which showed high rates of catalytic activity (438.3 U mg(-1)) and efficiently degraded saccharose (K(m)=6.4mM, V(max)=2.9 micromol saccharosemin(-1) and k(c)(at)=7.25 x 10(3)s(-1) at pH 4.9 and 37 degrees C). The invertase activity was strongly inhibited in a dose-dependent manner by SolyCIF produced in P. pastoris. In addition, Gel-SDS-PAGE analysis strongly suggests that TIV-1 was proteolyzed in planta and it was established that the fragments produced have to be tightly associated for its enzymatic activity to occur. We further investigated the location of the proteolytic sites by performing NH(2)-terminal Edman degradation on the fragments. The molecular model for TIV-1 shows that the fragmentation splits the catalytic site of the enzyme into two halves, which confirms that the enzymatic activity is possible only when the fragments are tightly associated.

摘要

蛋白质抑制剂是许多植物分泌的分子。在功能基因组学方法中,在茄科康奈尔大学数据库(www.sgn.cornell.edu)中鉴定出番茄的一种转化酶抑制剂(SolyCIF)。已确定该抑制剂主要在植物的叶、花和绿色果实中表达,并定位于细胞壁区室。通过进行RT-PCR克隆了SolyCIF cDNA,对其进行了全序列测定,并在毕赤酵母X-33中进行了异源表达。通过离子交换色谱和凝胶过滤获得的纯化重组蛋白进一步进行了生化表征,并用于进行亲和色谱。后一步使得纯化天然液泡转化酶(TIV-1)成为可能,该酶显示出高催化活性(438.3 U mg(-1)),并能有效降解蔗糖(在pH 4.9和37℃下,K(m)=6.4mM,V(max)=2.9微摩尔蔗糖分钟(-1),k(c)(at)=7.25×10(3)s(-1))。毕赤酵母产生的SolyCIF以剂量依赖性方式强烈抑制转化酶活性。此外,凝胶SDS-PAGE分析强烈表明TIV-1在植物中被蛋白酶解,并且已确定产生的片段必须紧密结合才能发生其酶活性。我们通过对片段进行氨基末端埃德曼降解进一步研究了蛋白水解位点的位置。TIV-1的分子模型表明,片段化将酶的催化位点分成两半,这证实只有当片段紧密结合时酶活性才可能发生。

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