摘要
将DSN(duplex-specific nuclease)均一化技术与SMART(switching mechanism at 5'end of RNA transcript)建库技术相结合,构建观音竹(Bambusa multiplex var.riviereorum)盐胁迫幼叶的均一化cDNA文库.经检测该原始文库滴度为1.7×106 cfu.mL-1,文库重组率达97%,插入片段的平均长度为1.5 kb.同时对文库中随机的600个单克隆进行测序,获得543个非重复序列,包括30个片段重叠群和513个单基因;文库冗余率为5.4%.表明观音竹盐胁迫幼叶均一化全长cDNA文库构建成功.
A normalized full-length cDNA library of the young leaf of Bambusa multiplex var.riviereorum was established by the method of DSN(duplex specific nuclease) normalization and SMART(switching mechanism at 5′end of RNA transcript).The titer of unamplified cDNA library was about 1.7×106 cfu·mL-1.The average size of cDNA inserts was 1500 bp with the recombination rate of 97%.Meanwhile a total of 543 unigenes were attained,including 30 contigs and 513 singltons by sequencing and analyzing 600 cDNA clones of normalized cDNA library.These results indicated that the normalized full-length cDNA library was established successfully.
出处
《福建农林大学学报(自然科学版)》
CSCD
北大核心
2012年第1期63-67,共5页
Journal of Fujian Agriculture and Forestry University:Natural Science Edition
基金
福建省科技厅资助项目(2009N0006
2011N5002)
关键词
观音竹
均一化
全长CDNA文库
盐胁迫
EST
Bambusa multiplex var.riviereorum
normalization
full-length cDNA library
salt stress
EST
