新型烟草花叶病毒外壳蛋白结晶方法的开发与应用。
The development and application of new crystallization method for tobacco mosaic virus coat protein.
机构信息
State Key Laboratory Breeding Base of Green Pesticide and Agricultural Bioengineering of Ministry of Education, Guizhou University, Huaxi District, Guiyang 550025, Guizhou Province, PR China.
出版信息
Virol J. 2012 Nov 21;9:279. doi: 10.1186/1743-422X-9-279.
BACKGROUND
Although tobacco mosaic virus (TMV) coat protein (CP) has been isolated from virus particles and its crystals have grown in ammonium sulfate buffers for many years, to date, no one has reported on the crystallization of recombinant TMV-CP connecting peptides expressed in E. coli.
METHODS
In the present papers genetically engineered TMV-CP was expressed, into which hexahistidine (His) tags or glutathione-S-transferase (GST) tags were incorporated. Considering that GST-tags are long peptides and His-tags are short peptides, an attempt was made to grow crystals of TMV-CP cleaved GST-tags (WT-TMV-CP32) and TMV-CP incorporated His-tags (WT-His-TMV-CP12) simultaneously in ammonium sulfate buffers and commercial crystallization reagents. It was found that the 20S disk form of WT-TMV-CP32 and WT-His-TMV-CP12 did not form high resolution crystals by using various crystallization buffers and commercial crystallization reagents. Subsequently, a new experimental method was adopted in which a range of truncated TMV-CP was constructed by removing several amino acids from the N- or the C-terminal, and high resolution crystals were grown in ammonium sulfate buffers and commercial crystallization reagents.
RESULTS
The new crystallization method was developed and 3.0 Å resolution macromolecular crystal was thereby obtained by removing four amino acids at the C-terminal of His-TMV-CP and connecting six His-tags at the N-terminal of His-TMV-CP (TR-His-TMV-CP19). The Four-layer aggregate disk structure of TR-His-TMV-CP19 was solved. This phenomenon showed that peptides at the C-terminus hindered the growth of high resolution crystals and the peptides interactions at the N-terminus were attributed to the quality of TMV-CP crystals.
CONCLUSION
A 3.0 Å resolution macromolecular crystal of TR-His-TMV-CP19 was obtained and the corresponding structure was solved by removing four amino acids at the C-terminus of TMV-CP and connecting His-tags at the N-terminus of TMV-CP. It indicated that short peptides influenced the resolution of TMV-CP crystals.
背景
尽管烟草花叶病毒(TMV)外壳蛋白(CP)已从病毒颗粒中分离出来,并在硫酸铵缓冲液中生长多年,但迄今为止,尚未有人报道过在大肠杆菌中表达的重组 TMV-CP 连接肽的结晶情况。
方法
本研究中,表达了经过基因工程改造的 TMV-CP,其中融合了六组氨酸(His)标签或谷胱甘肽 S-转移酶(GST)标签。考虑到 GST 标签是长肽,His 标签是短肽,因此尝试在硫酸铵缓冲液和商业结晶试剂中同时生长 GST 标签切割的 TMV-CP(WT-TMV-CP32)和 His 标签融合的 TMV-CP(WT-His-TMV-CP12)晶体。结果发现,使用各种结晶缓冲液和商业结晶试剂,20S 盘状 WT-TMV-CP32 和 WT-His-TMV-CP12 均无法形成高分辨率晶体。随后,采用了一种新的实验方法,通过从 N 端或 C 端去除几个氨基酸来构建一系列截短的 TMV-CP,并在硫酸铵缓冲液和商业结晶试剂中生长出高分辨率晶体。
结果
开发了新的结晶方法,通过去除 His-TMV-CP 的 C 端的四个氨基酸,并在 His-TMV-CP 的 N 端连接六个 His 标签,获得了分辨率为 3.0Å 的大分子晶体(TR-His-TMV-CP19)。解析了 TR-His-TMV-CP19 的四层聚集盘状结构。该现象表明,C 端的肽阻碍了高分辨率晶体的生长,而 N 端的肽相互作用归因于 TMV-CP 晶体的质量。
结论
通过去除 TMV-CP 的 C 端的四个氨基酸,并在 TMV-CP 的 N 端连接 His 标签,获得了分辨率为 3.0Å 的 TR-His-TMV-CP19 大分子晶体,并解析了相应的结构。这表明短肽影响 TMV-CP 晶体的分辨率。
Zotero 插件