The herpes simplex virus UL20 protein functions in glycoprotein K (gK) intracellular transport and virus-induced cell fusion are independent of UL20 functions in cytoplasmic virion envelopment

被引:0
作者
Jeffrey M Melancon
Preston A Fulmer
Konstantin G Kousoulas
机构
[1] Louisiana State University,Division of Biotechnology and Molecular Medicine, School of Veterinary Medicine
来源
Virology Journal | / 4卷
关键词
Intracellular Transport; Trans Golgi Network; UL20 Gene; Herpes Simplex Virus; Viral Plaque;
D O I
暂无
中图分类号
学科分类号
摘要
The HSV-1 UL20 protein (UL20p) and glycoprotein K (gK) are both important determinants of cytoplasmic virion morphogenesis and virus-induced cell fusion. In this manuscript, we examined the effect of UL20 mutations on the coordinate transport and Trans Golgi Network (TGN) localization of UL20p and gK, virus-induced cell fusion and infectious virus production. Deletion of 18 amino acids from the UL20p carboxyl terminus (UL20 mutant 204t) inhibited intracellular transport and cell-surface expression of both gK and UL20, resulting in accumulation of UL20p and gK in the endoplasmic reticulum (ER) in agreement with the inability of 204t to complement UL20-null virus replication and virus-induced cell fusion. In contrast, less severe carboxyl terminal deletions of either 11 or six amino acids (UL20 mutants 211t and 216t, respectively) allowed efficient UL20p and gK intracellular transport, cell-surface expression and TGN colocalization. However, while both 211t and 216t failed to complement for infectious virus production, 216t complemented for virus-induced cell fusion, but 211t did not. These results indicated that the carboxyl terminal six amino acids of UL20p were crucial for infectious virus production, but not involved in intracellular localization of UL20p/gK and concomitant virus-induced cell fusion. In the amino terminus of UL20, UL20p mutants were produced changing one or both of the Y38 and Y49 residues found within putative phosphorylation sites. UL20p tyrosine-modified mutants with both tyrosine residues changed enabled efficient intracellular transport and TGN localization of UL20p and gK, but failed to complement for either infectious virus production, or virus-induced cell fusion. These results show that UL20p functions in cytoplasmic envelopment are separable from UL20 functions in UL20p intracellular transport, cell surface expression and virus-induced cell fusion.
引用
收藏
相关论文
共 145 条
[1]  
Spear PG(1993)Entry of alphaherpesviruses into cells Seminars in Virology 4 167-180
[2]  
Spear PG(2004)Herpes simplex virus: receptors and ligands for cell entry Cell Microbiol 6 401-410
[3]  
Spear PG(2000)Three classes of cell surface receptors for alphaherpesvirus entry Virology 275 1-8
[4]  
Eisenberg RJ(2003)Herpesvirus entry: an update J Virol 77 10179-10185
[5]  
Cohen GH(2002)Herpesvirus assembly and egress J Virol 76 1537-1547
[6]  
Spear PG(2006)Herpesvirus assembly: a tale of two membranes Current opinion in microbiology 9 423-429
[7]  
Longnecker R(1991)The UL20 gene of herpes simplex virus 1 encodes a function necessary for viral egress J Virol 65 6414-6424
[8]  
Mettenleiter TC(1991)Investigation of herpes simplex virus type 1 genes encoding multiply inserted membrane proteins J Gen Virol 72 897-906
[9]  
Mettenleiter TC(1998)Importance of the herpes simplex virus UL24 gene for productive ganglionic infection in mice Virology 242 161-169
[10]  
Klupp BG(1982)Thymidine kinase deletion mutants of herpes simplex virus type 1 J Gen Virol 63 277-295
12345678910