大肠杆菌启动子文库的构建与基于模型的分析:代谢工程的必备工具
Construction and model-based analysis of a promoter library for E. coli: an indispensable tool for metabolic engineering.
作者信息
De Mey Marjan, Maertens Jo, Lequeux Gaspard J, Soetaert Wim K, Vandamme Erick J
机构信息
Department of Biochemical and Microbial Technology, Faculty of Bioscience Engineering, Ghent University, Coupure Links 653, Ghent, Belgium.
出版信息
BMC Biotechnol. 2007 Jun 18;7:34. doi: 10.1186/1472-6750-7-34.
BACKGROUND
Nowadays, the focus in metabolic engineering research is shifting from massive overexpression and inactivation of genes towards the model-based fine tuning of gene expression. In this context, the construction of a library of synthetic promoters of Escherichia coli as a useful tool for fine tuning gene expression is discussed here.
RESULTS
A degenerated oligonucleotide sequence that encodes consensus sequences for E. coli promoters separated by spacers of random sequences has been designed and synthesized. This 57 bp long sequence contains 24 conserved, 13 semi-conserved (W, R and D) and 20 random nucleotides. This mixture of DNA fragments was cloned into a promoter probing vector (pVIK165). The ligation mixtures were transformed into competent E. coli MA8 and the resulting clones were screened for GFP activity by measuring the relative fluorescence units; some clones produced high fluorescence intensity, others weak fluorescence intensity. The clones cover a range of promoter activities from 21.79 RFU/OD600 ml to 7606.83 RFU/OD600 ml. 57 promoters were sequenced and used for promoter analysis. The present results conclusively show that the postulates, which link promoter strength to anomalies in the -10 box and/or -35 box, and to the length of the spacer, are not generally valid. However, by applying Partial Least Squares regression, a model describing the promoter strength was built and validated.
CONCLUSION
For Escherichia coli, the promoter strength can not been linked to anomalies in the -10 box and/or -35 box, and to the length of the spacer. Also a probabilistic approach to relate the promoter sequence to its strength has some drawbacks. However, by applying Partial Least Squares regression, a good correlation was found between promoter sequence and promoter strength. This PLS model can be a useful tool to rationally design a suitable promoter in order to fine tune gene expression.
背景
如今,代谢工程研究的重点正从大量基因的过表达和失活转向基于模型的基因表达精细调控。在此背景下,本文讨论了构建大肠杆菌合成启动子文库作为精细调控基因表达的有用工具。
结果
设计并合成了一个简并寡核苷酸序列,该序列编码由随机序列间隔区隔开的大肠杆菌启动子共有序列。这个57bp长的序列包含24个保守核苷酸、13个半保守核苷酸(W、R和D)以及20个随机核苷酸。将该DNA片段混合物克隆到一个启动子探测载体(pVIK165)中。连接混合物转化到感受态大肠杆菌MA8中,通过测量相对荧光单位筛选所得克隆的绿色荧光蛋白(GFP)活性;一些克隆产生高荧光强度,另一些产生弱荧光强度。这些克隆的启动子活性范围为21.79 RFU/OD600 ml至7606.83 RFU/OD600 ml。对57个启动子进行了测序并用于启动子分析。目前的结果确凿地表明,将启动子强度与-10框和/或-35框中的异常以及间隔区长度联系起来的假设通常并不成立。然而,通过应用偏最小二乘回归,建立并验证了一个描述启动子强度的模型。
结论
对于大肠杆菌,启动子强度不能与-10框和/或-35框中的异常以及间隔区长度联系起来。此外,将启动子序列与其强度相关联的概率方法也存在一些缺陷。然而,通过应用偏最小二乘回归,发现启动子序列与启动子强度之间存在良好的相关性。这个偏最小二乘模型可以作为合理设计合适启动子以精细调控基因表达的有用工具。
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