Department of Microbiology and Infection Control, University Hospital of North Norway, Tromsø, Norway.
Metabolic and Renal Research Group, Department of Clinical Medicine, UiT-The Arctic University of Norway, Tromsø, Norway.
PLoS Pathog. 2024 Nov 21;20(11):e1012681. doi: 10.1371/journal.ppat.1012681. eCollection 2024 Nov.
BK polyomavirus (BKPyV) is a ubiquitous human virus that establishes a persistent infection in renal tubular epithelial cells and mainly causes disease in kidney transplant recipients. The closely related simian polyomavirus SV40 is known to cause cytoplasmic vacuolization in simian kidney cells, possibly increasing progeny release and cell death. This study aimed to determine whether BKPyV causes cytoplasmic vacuolization in primary human renal proximal tubule epithelial cells (RPTECs) and to investigate its potential role in the replication cycle. Using a large infectious dose (MOI 100-1000), a fraction of RPTECs (10-72%) showed early-wave vacuolization from 3 hours post-infection (hpi), which was mainly reversed by 36 hpi. Independent of the infectious dose, late-wave vacuolization occurred around the timepoint of progeny release. BKPyV receptor binding and internalization were required, as neuraminidase pretreatment and preincubation or treatment with a BKPyV-specific neutralizing antibody prevented early or late-occurring vacuolization. Microscopy revealed that the vacuoles were enlarged acidic endo-/lysosomal structures (dextran, EEA1, Rab5, Rab7, LAMP1, and/or Lysoview positive) that contained membrane-bound BKPyV. Time-lapse microscopy and quantitative PCR revealed that cell death and progeny release preceded late-wave vacuolization, mainly affecting cells directly neighboring the lysed cells. Thus, vacuolization had little impact on cell death or progeny release. Addition of the V-ATPase inhibitor Bafilomycin A1 at 0 hpi blocked vacuolization and BKPyV replication, but addition at 2 hpi only blocked vacuolization, suggesting that continuous endosomal acidification and maturation is needed for vacuole formation, but not for BKPyV replication. Our study shows that a massive uptake of BKPyV in RPTECs induces transient enlargement of endo-/lysosomes and is an early event in the viral replication cycle. Vacuolization gives no clear benefit for BKPyV and is possibly the result of a transiently overloaded endocytic pathway. Focal vacuolization around lysed cells suggests that the spread of BKPyV is preferably local.
BK 多瘤病毒(BKPyV)是一种普遍存在的人类病毒,在肾小管上皮细胞中建立持续性感染,主要导致肾移植受者发病。密切相关的猿猴多瘤病毒 SV40 已知会导致猿猴肾细胞中的细胞质空泡化,可能会增加后代释放和细胞死亡。本研究旨在确定 BKPyV 是否会导致原代人肾近端小管上皮细胞(RPTEC)中的细胞质空泡化,并研究其在复制周期中的潜在作用。使用大感染剂量(MOI100-1000),一部分 RPTEC(10-72%)在感染后 3 小时(hpi)显示早期波空泡化,主要在 36 hpi 时逆转。与感染剂量无关,晚期波空泡化发生在后代释放的时间点附近。BKPyV 受体结合和内化是必需的,因为神经氨酸酶预处理和预孵育或用 BKPyV 特异性中和抗体处理可防止早期或晚期发生空泡化。显微镜观察显示,空泡是扩大的酸性内体/溶酶体结构(葡聚糖、EEA1、Rab5、Rab7、LAMP1 和/或 Lysoview 阳性),其中包含膜结合的 BKPyV。延时显微镜和定量 PCR 显示,细胞死亡和后代释放先于晚期空泡化,主要影响直接邻近裂解细胞的细胞。因此,空泡化对细胞死亡或后代释放影响不大。在 0 hpi 添加 V-ATP 酶抑制剂巴弗洛霉素 A1 可阻断空泡化和 BKPyV 复制,但在 2 hpi 添加仅阻断空泡化,表明持续的内体酸化和成熟是形成空泡所必需的,但不是 BKPyV 复制所必需的。我们的研究表明,大量 BKPyV 在 RPTEC 中的摄取会导致内体/溶酶体的短暂扩大,这是病毒复制周期中的早期事件。空泡化对 BKPyV 没有明显的益处,可能是暂时超载的内吞途径的结果。在裂解细胞周围出现局灶性空泡化表明 BKPyV 的传播更倾向于局部。
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