首页> 美国卫生研究院文献>Journal of Virology >Dual Functions of Bacteriophage T4D Gene 28 Product: Structural Component of the Viral Tail Baseplate Central Plug and Cleavage Enzyme for Folyl Polyglutamates I. Identification of T4D Gene 28 Product in the Tail Plug
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Dual Functions of Bacteriophage T4D Gene 28 Product: Structural Component of the Viral Tail Baseplate Central Plug and Cleavage Enzyme for Folyl Polyglutamates I. Identification of T4D Gene 28 Product in the Tail Plug

机译:噬菌体T4D基因28产品的双重功能:病毒尾底板中央塞的结构成分和聚谷氨酸叶酸酯的切割酶I.尾塞中T4D基因28产品的鉴定

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摘要

The T4D bacteriophage gene 28 product is a component of the central plug of the tail baseplate, as shown by the following two independent lines of evidence. (i) A highly sensitive method for radioactive labeling of only tail baseplate plug components was developed. These labeled plug components were incorporated by a complementation procedure into new phage particles and were analyzed by radioautography after sodium dodecyl sulfate-polyacrylamide gel electrophoresis. Three new structural proteins were found in addition to the three known tail plug proteins (i.e., gP29, gP27, and gP5). One of the three newly identified components had a molecular weight of 24,000 to 25,000 and appeared to be a product of T4D gene 28. (ii) Characterization of mutants of Escherichia coli bacteriophage T4D which produced altered gene 28 products also indicated that the gene 28 product was a viral tail component. T4D 28ts phage particles produced at the permissive temperature had altered heat labilities compared with parent T4D particles. We isolated a single-step temperature revertant of T4D 28ts and found that it produced phage particles which phenotypically resembled the original T4D particles. Since the properties of the phage baseplate components usually determine heat lability, these two changes in physical stability after two sequential single mutations in gene 28 supported the other evidence that the gene 28 product was a viral baseplate component. Also, compared with parent T4D particles, T4D 28ts and T4D 28am viral particles adsorbed at different rates to various types of host cells. In addition, T4D 28ts particles exhibited a different host range than parent T4D particles. This T4D mutant formed plaques with an extremely low efficiency on all E. coli K-12 strains tested. We found that although T4D 28ts particles adsorbed rapidly and irreversibly to the E. coli K-12 strains, as judged by gene rescue experiments, these particles were not able to inject their DNA into the E. coli K-12 strains. On the other hand, the T4D 28ts revertant had a plating efficiency on E. coli K-12 strains that was quite similar to the plating efficiency of the original parent, T4D. These properties of phage particles containing an altered gene 28 product supported the analytical finding that the gene 28 product is a structural component of the central plug of the T4D tail baseplate. They also indicated that this component plays a role in both host cell recognition and viral DNA injection.
机译:T4D噬菌体基因28产物是尾巴底板中央栓塞的组成部分,如以下两条独立的证据所示。 (i)开发了一种仅对尾底板塞组件进行放射性标记的高灵敏度方法。通过补充程序将这些标记的塞子组分掺入新的噬菌体颗粒中,并在十二烷基硫酸钠-聚丙烯酰胺凝胶电泳后通过放射自显影分析。除了三个已知的尾塞蛋白(即gP29,gP27和gP5)之外,还发现了三个新的结构蛋白。新鉴定出的三个成分之一的分子量为24,000至25,000,似乎是T4D基因28的产物。(ii)表征产生改变的基因28产物的大肠杆菌噬菌体T4D突变体也表明该基因28产物是病毒尾巴成分。与母体T4D颗粒相比,在许可温度下产生的T4D 28 ts 噬菌体颗粒具有改变的热不稳定性。我们分离出T4D 28 ts 的单步温度回复剂,发现它产生的噬菌体颗粒在表型上与原始T4D颗粒相似。由于噬菌体基板成分的特性通常决定了热稳定性,因此在基因28中出现两个连续的单次突变后,这两个物理稳定性的变化支持了另一种证据,证明基因28产物是病毒基板成分。而且,与亲本T4D颗粒相比,T4D 28 ts 和T4D 28am病毒颗粒以不同的速率吸附到各种类型的宿主细胞上。另外,T4D 28 ts 颗粒与母体T4D颗粒表现出不同的宿主范围。该T4D突变体在所有测试的大肠杆菌K-12菌株上形成极低效率的噬菌斑。我们发现,尽管通过基因拯救实验判断,T4D 28 ts 颗粒迅速且不可逆地吸附到大肠杆菌K-12菌株中,但这些颗粒无法将其DNA注入大肠杆菌中。 K-12株。另一方面,T4D 28 ts 还原剂在大肠杆菌K-12菌株上的平板接种效率与原始亲本T4D的平板接种效率非常相似。包含改变的基因28产物的噬菌体颗粒的这些特性支持了分析发现,即基因28产物是T4D尾部底板的中央栓塞的结构成分。他们还指出,该成分在宿主细胞识别和病毒DNA注射中均起着作用。

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