首页> 外文期刊>FEMS Microbiology Letters >Promoters of crystal protein genes do not control crystal formation inside exosporium of Bacillus thuringiensis ssp finitimus strain YBT-020
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Promoters of crystal protein genes do not control crystal formation inside exosporium of Bacillus thuringiensis ssp finitimus strain YBT-020

机译:晶体蛋白基因的启动子不能控制苏云金芽孢杆菌ssp finitimus菌株YBT-020的孢子囊内的晶体形成

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摘要

Most Bacillus thuringiensis parasporal crystals separate from spores after sporulation. A special phenomenon called spore-crystal association (SCA) occurs in a few subspecies (e.g. ssp. finitimus) where enclosed crystals are associated with spores. In this study, the involvement of crystal protein gene promoters in SCA was investigated. Two crystal protein genes, cry26Aa and cry28Aa, were isolated from subspecies finitimus strain YBT-020, and each or both were then transferred to acrystalliferous B. thuringiensis strain BMB171 and the plasmid-cured derivative of strain YBT-020. SCA was not observed with any recombinant strain, implying that the crystal protein genes are not sufficient to cause SCA. When the typical crystal protein gene cry1Ca was introduced into strain YBT-020, free bipyramidal crystals formed in addition to SCA. Recombinant genes containing the promoter of cry26Aa or cry28Aa fused with the coding sequence (CDS) of cry1Ca were introduced into strain YBT-020, and the typical cry1Ca phenotype was observed. Another two fusion genes consisting of the promoter of cry1Ca and the CDS of cry26Aa or cry28Aa were also transferred to strain YBT-020. Only enclosed crystals formed. These results indicate that the promoters of the crystal protein genes are not the key factor determining the crystal location in strain YBT-020.
机译:苏云金芽孢杆菌大多数孢子体形成孢子后从孢子中分离出来。在少数亚种(例如ssp.finitimus)中会出现一种称为孢子-晶体缔合(SCA)的特殊现象,其中封闭的晶体与孢子有关。在这项研究中,研究了晶体蛋白基因启动子在SCA中的参与。从亚种finitimus菌株YBT-020中分离了两个晶体蛋白基因cry26Aa和cry28Aa,然后将每一个或全部转移到苏云金芽胞杆菌结晶菌株BMB171和质粒固化菌株YBT-020的衍生物中。在任何重组菌株中均未观察到SCA,这表明晶体蛋白基因不足以引起SCA。当将典型的晶体蛋白基因cry1Ca引入菌株YBT-020时,除SCA外还形成了游离的双锥体晶体。将含有与cry1Ca的编码序列(CDS)融合的cry26Aa或cry28Aa启动子的重组基因引入菌株YBT-020,并观察到典型的cry1Ca表型。由cry1Ca的启动子和cry26Aa或cry28Aa的CDS组成的另外两个融合基因也被转移到YBT-020菌株中。仅形成封闭的晶体。这些结果表明,晶体蛋白基因的启动子不是决定菌株YBT-020中晶体位置的关键因素。

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