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| Moclecular Cloning and Sequence Analysis of SPT Gene Transcription Factor
Regulation of Pistil from Cabbage |
| YANG Pu-li,XU Jun-qiang,LIU Zhi-yu,WANG Zhi-min,ZHANG Dan-hua,TANG Qing-lin*,
SONG Ming* |
College of Horticulture and Landscape Architecture, Southwest University, Key Laboratory of Horticulture Science for
Southern Mountainous Regions, Ministry of Education, Key Laboratory of Olericulture, Chongqing 400715, China |
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Abstract Taking cabbage(Brassica oleracea L.) E1 as materials,We extracted total RNA
from capullo,reverse transcribed cDNA. According to SPT gene sequence of Arabidopsis,primers
were designed and 1 085 bp SPT gene with 1 062 bp open reading frame(ORF)was cloned by homology
cloning techniques. The deduced BoSPT protein contained 353 amino acids,with a molecular
weight of 37.67 kD and pI of 6.83. After double enzyme of EcoRI and KpnI restriction enzymes,
and then construct the recombinant plasmids pET43.1a-BoSPT. After transformation to E. coli Rosetta(
DE3),the expression of recombinant proteins were detected via SDS-PAGE. The structural
analysis of BoSPT though Smart-embl showed that it contained bHLH family domain,which located
at the position of 173-221 amino acid residues,The phylogenetic tree indicated that the BoSPT had close genetic relationship with AtSPT and AlSPT. Prokaryotic expression showed that the molecular
mass of BoSPT protein was purified.
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Received: 22 June 2013
Published: 14 August 2013
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