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利用新型 PCR 引物系统检测苏云金芽孢杆菌的新 cry 基因。

Detection of new cry genes of Bacillus thuringiensis by use of a novel PCR primer system.

机构信息

Departamento de Biotecnologia y Bioquimica, CINVESTAV, 36500 Irapuato, Gto., Mexico.

出版信息

Appl Environ Microbiol. 2010 Sep;76(18):6150-5. doi: 10.1128/AEM.00797-10. Epub 2010 Jul 23.

Abstract

On the basis of the known cry gene sequences of Bacillus thuringiensis, three sets of primers were designed from four conserved blocks found in the delta-endotoxin-coding region. The primer pairs designed amplify the regions between blocks 1 and 5, 2 and 5, and 1 and 4. In silico analyses indicated that 100% of the known three-domain cry gene sequences can be amplified by these sets of primers. To test their ability to amplify known and unknown cry gene sequences, 27 strains from the CINVESTAV (LBIT series) collection showing atypical crystal morphology were selected. Their DNA was used as the template with the new primer system, and after a systematic amplification and sequencing of the amplicons, each strain showed one or more cry-related sequences, totaling 54 different sequences harbored by the 27 strains. Seven sequences were selected on the basis of their low level of identity to the known cry sequences, and once cloning and sequencing of the complete open reading frames were done, three new cry-type genes (primary ranks) were identified and the toxins that they encode were designated Cry57Aa1, Cry58Aa1, and Cry59Aa1 by the B. thuringiensis Toxin Nomenclature Committee. The rest of the seven sequences were classified Cry8Ka2, Cry8-like, Cry20Ba1, and Cry1Ma1 by the committee. The crystal morphology of the selected strains and analysis of the new Cry protein sequences showed interesting peculiarities.

摘要

基于苏云金芽孢杆菌已知的 cry 基因序列,从编码δ-内毒素的区域中发现的四个保守块设计了三组引物。设计的引物对扩增了 1 和 5 块、2 和 5 块以及 1 和 4 块之间的区域。计算机分析表明,这些引物组可以扩增 100%已知的三域 cry 基因序列。为了测试它们扩增已知和未知 cry 基因序列的能力,选择了来自 CINVESTAV(LBIT 系列)收集的 27 株表现出非典型晶体形态的菌株。用新的引物系统以它们的 DNA 为模板进行系统扩增和测序,每个菌株都显示出一个或多个与 cry 相关的序列,27 株菌共携带 54 个不同的序列。根据它们与已知 cry 序列的低同一性,选择了七个序列,一旦完成完整开放阅读框的克隆和测序,就鉴定了三个新的 cry 型基因(主要等级),并由苏云金芽孢杆菌毒素命名委员会将它们编码的毒素指定为 Cry57Aa1、Cry58Aa1 和 Cry59Aa1。其余的七个序列被委员会分类为 Cry8Ka2、Cry8-like、Cry20Ba1 和 Cry1Ma1。所选菌株的晶体形态和新 Cry 蛋白序列分析显示出有趣的特点。

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