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出 处:《南开大学学报(自然科学版)》1998年第1期64-71,共8页Acta Scientiarum Naturalium Universitatis Nankaiensis
摘 要:以E.coli质粒pJRD184为基础,将多酶切点引入地衣芽胞杆菌(Bacilluslicheniformis)的a-淀粉酶基因信号肽编码区的PstI切点,构建了能表达并将a-淀粉酶(Amy)渗漏到胞外的E.coli克隆载体pLAM9712.该载体可根据在含有可溶性淀粉的LB平板上菌落周围有没有淀粉水解圈直接筛选重组子,从而避免了使用异丙基硫代-β-D-半乳糖苷(IPTG)、5-溴-4-氯-3-吲哚-β-D一半乳糖苷(X-gal),代之以廉价的碘、淀粉.实验进一步验证了pLAM9712在基因克隆中的可行性及质粒本身的稳定性.Based on pJRD184, an E. coli cloning vector pLAM9172 has been constructed by inserting MCS into PstI restriction site of signal sequence coding region of a-amylase gene from Bacillus lichenlers. It prossesses the advantage over existing E. coli cloning vectors: Directly screening the recombinants on LBS plates by the loss of the hola around the colonies, inexpensive indicators, iodine/starch, instead of the very expensive ones, IPTG/X-gal; Furthermore, it has been proved that the cloning vector is not only stable in E. coli but also available in gene cloning.
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