Molecular cloning and characterization of the CHS gene family in turmeric (Curcuma longa Linn.)

被引:0
|
作者
Sirinrat Wannapinpong
Kornsorn Srikulnath
Amara Thongpan
Kiattawee Choowongkomon
Surin Peyachoknagul
机构
[1] Kasetsart University,Department of Genetics, Faculty of Science
[2] Center for Advanced Studies in Tropical Natural Resources,Institute of Food Research and Product Development
[3] National Research University-Kasetsart University,Laboratory of Animal Cytogenetics and Comparative Genomics, Department of Genetics, Faculty of Science
[4] (CASTNAR,Department of Biochemistry, Faculty of Science
[5] NRU-KU),undefined
[6] Kasetsart University,undefined
[7] Kasetsart University,undefined
[8] Kasetsart University,undefined
来源
Journal of Plant Biochemistry and Biotechnology | 2015年 / 24卷
关键词
CHS; Gene family; TAIL-PCR; Molecular docking; Turmeric;
D O I
暂无
中图分类号
学科分类号
摘要
Three chalcone synthase (CHS) genes were isolated from Curcuma longa Linn. using TAIL-PCR. ClCHS1 and ClCHS2 were 1,460 and 1,407 bp in length, respectively, containing 1,191 bp open reading frame (ORF) that encodes 396 amino acids, whereas ClCHS3 was 1,394 bp in length containing 1,170 bp ORF that encodes 389 amino acids. The structure of all three genes comprise two exons and one intron which are consistent with the other CHS gene family. Southern blot analysis using a ClCHS conserved fragment revealed the ClCHS genes belong to a gene family. Phylogenetic analysis showed the three putative ClCHS proteins to be closely related to DCS (diketide-CoA synthase) protein, a product of CHS-like gene in C. longa, which condenses malonyl-CoA with feruloyl-CoA or coumaroyl-CoA as the substrate in curcuminoid synthesis. These results suggest that the interaction of substrate and enzyme between the three putative ClCHS proteins and DCS might be highly similar. Homology modeling and docking analysis were consistent, indicating that the same substrate (coumaroyl-CoA) can be used in the putative ClCHS1 and ClCHS2 proteins. However, the putative ClCHS3 protein seems to have seven amino acids deletion in a loop involved in the binding site formation, suggesting that the binding site with coumaroyl-CoA might be altered.
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页码:25 / 33
页数:8
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