摘要
本文从罗布麻(Apocynumvenetum)幼苗中提取了大分子量DNA,经Sau3A部分酶解,从琼脂糖凝胶中回收12-22kb的"目的"DNA片段,用BamHI/EcoRI双酶切入EMBL3DNA制备克隆载体。"目的"DNA片段与载体连接,体外包装,所得重组子数为3.74×106pfu,达到了建库要求的理论值。以番茄1,5-二磷酸核酮糖羧化酶/加氧酶(Rubisco)小亚基基因(rbcS)的cDNA为探针,用噬菌斑原位杂交法,斑点杂交法,从基因文库中选出4个含罗布麻rbcS基因的阳性克隆。
Vector DNA was prepared by double digestion of λEMBL3 DNA withBamHI / EcoRI. High molecular weight dogbane (Apocynum Venetum) was isolated frometiolated shoots and partially digested with San 3A. The dogbane insert DNA fragementswith the size of 12-22 kb were recovered from agarose gel and joined with theEMBL3 vectors. The recombinant molecules were packaged into viable phage particles invitro and the yield of recombinant phages was 3.74 × 106 pfu. This figure met with the theoretical value required for dogbane genomic library. The library was screened by using theprob of tomato rbc S-2 cDNA. Four positive clones were obtained.
出处
《山东农业大学学报(自然科学版)》
CSCD
1995年第1期8-12,共5页
Journal of Shandong Agricultural University:Natural Science Edition
关键词
罗布麻
基因文库
RUBISCO
dogbane
genetic library
small subunit of ribulose 1,5-bisphosphatecarboxylase / oxygenase
