Fomenkov Alexey, Sun Zhiyi, Dila Deborah K, Anton Brian P, Roberts Richard J, Raleigh Elisabeth A
Research Department, New England Biolabs, Ipswich, MA, United States of America.
PLoS One. 2017 Jun 27;12(6):e0179853. doi: 10.1371/journal.pone.0179853. eCollection 2017.
Here we characterize the modification-dependent restriction enzyme (MDE) EcoBLMcrX in vivo, in vitro and in its genomic environment. MDE cleavage of modified DNAs protects prokaryote populations from lethal infection by bacteriophage with highly modified DNA, and also stabilizes lineages by reducing gene import when sparse modification occurs in the wrong context. The function and distribution of MDE families are thus important. Here we describe the properties of EcoBLMcrX, an enzyme of the E. coli B lineage, in vivo and in vitro. Restriction in vivo and the genome location of its gene, ecoBLmcrX, were determined during construction and sequencing of a B/K-12 hybrid, ER2566. In classical restriction literature, this B system was named r6 or rglAB. Like many genome defense functions, ecoBLmcrX is found within a genomic island, where gene content is variable among natural E. coli isolates. In vitro, EcoBLMcrX was compared with two related enzymes, BceYI and NhoI. All three degrade fully cytosine-modified phage DNA, as expected for EcoBLMcrX from classical T4 genetic data. A new method of characterizing MDE specificity was developed to better understand action on fully-modified targets such as the phage that provide major evolutionary pressure for MDE maintenance. These enzymes also cleave plasmids with m5C in particular motifs, consistent with a role in lineage-stabilization. The recognition sites were characterized using a site-ranking approach that allows visualization of preferred cleavage sites when fully-modified substrates are digested. A technical constraint on the method is that ligation of one-nucleotide 5' extensions favors G:C over A:T approximately five-fold. Taking this bias into account, we conclude that EcoBLMcrX can cleave 3' to the modified base in the motif Rm5C|. This is compatible with, but less specific than, the site reported by others. Highly-modified site contexts, such as those found in base-substituted virulent phages, are strongly preferred.
在此,我们在体内、体外及其基因组环境中对修饰依赖性限制酶(MDE)EcoBLMcrX进行了表征。修饰DNA的MDE切割可保护原核生物群体免受携带高度修饰DNA的噬菌体的致命感染,并且当在错误的背景下发生稀疏修饰时,还可通过减少基因导入来稳定谱系。因此,MDE家族的功能和分布很重要。在此,我们描述了大肠杆菌B谱系的一种酶EcoBLMcrX在体内和体外的特性。在构建和测序B/K-12杂交菌株ER2566的过程中,确定了其在体内的限制作用及其基因ecoBLmcrX的基因组位置。在经典的限制文献中,这个B系统被命名为r6或rglAB。与许多基因组防御功能一样,ecoBLmcrX存在于一个基因组岛中,在天然大肠杆菌分离株中基因含量是可变的。在体外,将EcoBLMcrX与两种相关酶BceYI和NhoI进行了比较。正如根据经典T4遗传数据对EcoBLMcrX的预期那样,这三种酶都能降解完全胞嘧啶修饰的噬菌体DNA。为了更好地理解对完全修饰的靶标的作用,开发了一种表征MDE特异性的新方法,这些靶标例如为MDE维持提供主要进化压力的噬菌体。这些酶还能切割特定基序中带有m5C的质粒,这与它们在谱系稳定中的作用一致。使用位点排序方法对识别位点进行了表征,该方法允许在消化完全修饰的底物时可视化优选的切割位点。该方法的一个技术限制是,单核苷酸5' 延伸的连接对G:C的偏好比对A:T大约高五倍。考虑到这种偏差,我们得出结论,EcoBLMcrX可以在基序Rm5C|中修饰碱基的3' 端进行切割。这与其他人报道的位点相符,但特异性较低。高度修饰的位点背景,例如在碱基取代的烈性噬菌体中发现的那些,是强烈优选的。
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