Cre- lox -Based System for Multiple Gene Deletions and Selectable-Marker Removal in Lactobacillus plantarum

生物 可选择标记 重组酶 遗传学 Cre重组酶 基因 突变体 Cre-Lox重组 同源重组 突变 基因盒 穿梭机载体 SOS响应 重组工程 表情盒 基因靶向 位点特异性重组 质粒 载体(分子生物学) 转基因 重组 重组DNA 转基因小鼠 整合子
作者
Jolanda Lambert,Roger S. Bongers,Michiel Kleerebezem
出处
期刊:Applied and Environmental Microbiology [American Society for Microbiology]
卷期号:73 (4): 1126-1135 被引量:228
标识
DOI:10.1128/aem.01473-06
摘要

The classic strategy to achieve gene deletion variants is based on double-crossover integration of nonreplicating vectors into the genome. In addition, recombination systems such as Cre-lox have been used extensively, mainly for eukaryotic organisms. This study presents the construction of a Cre-lox-based system for multiple gene deletions in Lactobacillus plantarum that could be adapted for use on gram-positive bacteria. First, an effective mutagenesis vector (pNZ5319) was constructed that allows direct cloning of blunt-end PCR products representing homologous recombination target regions. Using this mutagenesis vector, double-crossover gene replacement mutants could be readily selected based on their antibiotic resistance phenotype. In the resulting mutants, the target gene is replaced by a lox66-P(32)-cat-lox71 cassette, where lox66 and lox71 are mutant variants of loxP and P(32)-cat is a chloramphenicol resistance cassette. The lox sites serve as recognition sites for the Cre enzyme, a protein that belongs to the integrase family of site-specific recombinases. Thus, transient Cre recombinase expression in double-crossover mutants leads to recombination of the lox66-P(32)-cat-lox71 cassette into a double-mutant loxP site, called lox72, which displays strongly reduced recognition by Cre. The effectiveness of the Cre-lox-based strategy for multiple gene deletions was demonstrated by construction of both single and double gene deletions at the melA and bsh1 loci on the chromosome of the gram-positive model organism Lactobacillus plantarum WCFS1. Furthermore, the efficiency of the Cre-lox-based system in multiple gene replacements was determined by successive mutagenesis of the genetically closely linked loci melA and lacS2 in L. plantarum WCFS1. The fact that 99.4% of the clones that were analyzed had undergone correct Cre-lox resolution emphasizes the suitability of the system described here for multiple gene replacement and deletion strategies in a single genetic background.
最长约 10秒,即可获得该文献文件

科研通智能强力驱动
Strongly Powered by AbleSci AI
科研通是完全免费的文献互助平台,具备全网最快的应助速度,最高的求助完成率。 对每一个文献求助,科研通都将尽心尽力,给求助人一个满意的交代。
实时播报
哈哈哈完成签到,获得积分10
刚刚
CuCd发布了新的文献求助10
刚刚
开放夏蓉发布了新的文献求助10
1秒前
小二郎应助Aletheia采纳,获得10
1秒前
西蓝花发布了新的文献求助10
1秒前
Arron发布了新的文献求助10
1秒前
脑洞疼应助YY采纳,获得10
1秒前
若菲发布了新的文献求助10
2秒前
EinZwei发布了新的文献求助10
2秒前
2秒前
无情的麦片完成签到,获得积分10
2秒前
4秒前
kk完成签到,获得积分10
4秒前
华仔应助qq采纳,获得10
4秒前
伶俐妙海应助迟归采纳,获得20
5秒前
李善聪发布了新的文献求助10
5秒前
柚子发布了新的文献求助10
5秒前
6秒前
奕崽发布了新的文献求助10
6秒前
英勇的铸海完成签到,获得积分10
6秒前
宫爆机顶关注了科研通微信公众号
6秒前
香蕉觅云应助wu采纳,获得10
7秒前
无辜的雪曼完成签到 ,获得积分20
7秒前
wp4605应助zzx采纳,获得60
7秒前
Savannah发布了新的文献求助10
8秒前
8秒前
青柚发布了新的文献求助20
9秒前
Vincent发布了新的文献求助10
10秒前
非我发布了新的文献求助10
10秒前
tiana完成签到,获得积分10
10秒前
11秒前
852应助蜗牛采纳,获得10
11秒前
顾矜应助尚中庸采纳,获得10
11秒前
aa关注了科研通微信公众号
12秒前
12秒前
12秒前
未来123发布了新的文献求助30
12秒前
福福完成签到,获得积分10
12秒前
jiangjiarui应助jinyu采纳,获得10
13秒前
oia完成签到,获得积分10
13秒前
高分求助中
Principles of Economics, 11th Edition 10000
University Physics with Modern Physics, 16th edition 10000
(应助此贴封号)【重要!!请各用户(尤其是新用户)详细阅读】【科研通的精品贴汇总】 10000
Arthritis and Related Conditions, An Issue of Orthopedic Clinics 1000
Development of a Bridge Weigh-In-Motion System: A technology to convert the bridge response to the passage of traffic into data on vehicle configurations, speeds, times of travel and weights 1000
ズームレンズの光学設計に関する研究 800
Fundamentals of Pharmaceutical and Biologics Regulations: A Global Perspective, Second Edition 700
热门求助领域 (近24小时)
化学 材料科学 医学 生物 纳米技术 工程类 有机化学 化学工程 生物化学 计算机科学 内科学 物理 复合材料 催化作用 细胞生物学 无机化学 光电子学 物理化学 电极 基因
热门帖子
关注 科研通微信公众号,转发送积分 7285944
求助须知:如何正确求助?哪些是违规求助? 8906401
关于积分的说明 18847149
捐赠科研通 6955567
什么是DOI,文献DOI怎么找? 3208231
关于科研通互助平台的介绍 2378354
邀请新用户注册赠送积分活动 2183853