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本文引用的文献

1
Mutations in the BC-loop of the BKV VP1 region do not influence viral load in renal transplant patients.BK病毒VP1区域BC环的突变不影响肾移植患者的病毒载量。
J Med Virol. 2009 Jan;81(1):75-81. doi: 10.1002/jmv.21359.
2
Polyomavirus BK with rearranged noncoding control region emerge in vivo in renal transplant patients and increase viral replication and cytopathology.具有重排非编码控制区的多瘤病毒BK在肾移植患者体内出现,并增加病毒复制和细胞病理学变化。
J Exp Med. 2008 Apr 14;205(4):841-52. doi: 10.1084/jem.20072097. Epub 2008 Mar 17.
3
Identification of amino acid residues in BK virus VP1 that are critical for viability and growth.鉴定BK病毒VP1中对病毒存活和生长至关重要的氨基酸残基。
J Virol. 2007 Nov;81(21):11798-808. doi: 10.1128/JVI.01316-07. Epub 2007 Aug 15.
4
Even distribution of BK polyomavirus subtypes and subgroups in the Japanese Archipelago.BK多瘤病毒亚型和亚组在日本列岛的分布情况
Arch Virol. 2007;152(9):1613-21. doi: 10.1007/s00705-007-0997-y. Epub 2007 Jun 1.
5
Relationships between BK virus lineages and human populations.BK病毒谱系与人类群体之间的关系。
Microbes Infect. 2007 Feb;9(2):204-13. doi: 10.1016/j.micinf.2006.11.008. Epub 2006 Dec 8.
6
Identification of a genomic subgroup of BK polyomavirus spread in European populations.BK多瘤病毒在欧洲人群中传播的一个基因组亚群的鉴定。
J Gen Virol. 2006 Nov;87(Pt 11):3201-3208. doi: 10.1099/vir.0.82266-0.
7
Evolution of BK virus based on complete genome data.基于全基因组数据的BK病毒进化
J Mol Evol. 2006 Sep;63(3):341-52. doi: 10.1007/s00239-005-0092-5. Epub 2006 Jul 28.
8
Genetic variability in BK Virus regulatory regions in urine and kidney biopsies from renal-transplant patients.肾移植患者尿液和肾活检组织中BK病毒调控区的基因变异性。
J Med Virol. 2006 Mar;78(3):384-93. doi: 10.1002/jmv.20551.
9
BK virus regulatory region sequence deletions in a case of human polyomavirus associated nephropathy (PVAN) after kidney transplantation.肾移植后人类多瘤病毒相关性肾病(PVAN)一例中BK病毒调控区序列缺失
J Clin Virol. 2006 Jan;35(1):106-8. doi: 10.1016/j.jcv.2005.08.003. Epub 2005 Sep 30.
10
A prospective longitudinal study of BK virus infection in 104 renal transplant recipients.一项对104名肾移植受者进行的BK病毒感染前瞻性纵向研究。
Am J Transplant. 2005 Aug;5(8):1926-33. doi: 10.1111/j.1600-6143.2005.00934.x.

肾移植受者中BK病毒VP1外环的突变与尿液病毒载量

Mutations in the external loops of BK virus VP1 and urine viral load in renal transplant recipients.

作者信息

Tremolada Sara, Delbue Serena, Castagnoli Lorenzo, Allegrini Sara, Miglio Umberto, Boldorini Renzo, Elia Francesca, Gordon Jennifer, Ferrante Pasquale

机构信息

Department of Public Health-Microbiology-Virology, University of Milan, Milan, Italy.

出版信息

J Cell Physiol. 2010 Jan;222(1):195-9. doi: 10.1002/jcp.21937.

DOI:10.1002/jcp.21937
PMID:19780025
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2783606/
Abstract

Polyomavirus-associated nephropathy (PVAN) is a major complication that occurs after renal transplantation and is induced by reactivation of the human polyomavirus BK (BKV). The structure of the viral capsid protein 1 (VP1) is characterized by the presence of external loops, BC, DE, EF, GH, and HI, which are involved in receptor binding. The pathogenesis of PVAN is not well understood, but viral risk factors are thought to play a crucial role in the onset of this pathology. In an attempt to better understand PVAN pathogenesis, the BKV-VP1 coding region was amplified, cloned, and sequenced from the urine of kidney transplant recipients who did, and did not, develop the pathology. Urine viral loads were determined by using real time quantitative PCR (Q-PCR). Amino acid substitutions were detected in 6/8 patients, and 6/7 controls. The BC and EF loop regions were most frequently affected by mutations, while no mutations were found within the GH and HI loops of both patients and controls. Some mutations, that were exclusively detected in the urine of PVAN patients, overlapped with previously reported mutations, although a correlation between changes in amino acids and the development of PVAN was not found. Urine viral loads were higher than that of the proposed cut-off loads for identification of patients that are at a high risk of developing PVAN (10(7) copies/ml), both in the PVAN and control groups, thus confirming that urine viral load is not a useful predictive marker for the development of PVAN.

摘要

多瘤病毒相关性肾病(PVAN)是肾移植后发生的一种主要并发症,由人多瘤病毒BK(BKV)重新激活所致。病毒衣壳蛋白1(VP1)的结构特点是存在外部环,即BC、DE、EF、GH和HI环,这些环参与受体结合。PVAN的发病机制尚不完全清楚,但病毒危险因素被认为在这种病理状态的发生中起关键作用。为了更好地理解PVAN的发病机制,从发生和未发生该病理状态的肾移植受者尿液中扩增、克隆并测序了BKV-VP1编码区。通过实时定量PCR(Q-PCR)测定尿液病毒载量。在8例患者中的6例以及7例对照中检测到氨基酸替换。BC环和EF环区域最常受到突变影响,而在患者和对照的GH环和HI环内均未发现突变。一些仅在PVAN患者尿液中检测到的突变与先前报道的突变重叠,尽管未发现氨基酸变化与PVAN发生之间的相关性。PVAN组和对照组的尿液病毒载量均高于用于识别有高风险发生PVAN患者的建议临界载量(10⁷拷贝/ml),因此证实尿液病毒载量不是PVAN发生的有用预测标志物。