Orandle M S, Papadi G P, Bubenik L J, Dailey C I, Johnson C M
Department of Pathobiology, University of Florida, Gainesville 32610, USA.
AIDS Res Hum Retroviruses. 1997 May 1;13(7):611-20. doi: 10.1089/aid.1997.13.611.
Thymus alterations associated with feline immunodeficiency virus (FIV), an AIDS animal model, were investigated by measuring phenotypic composition of thymocytes, structure of thymic epithelial cells, and transcription of viral RNA in the thymus of FIV-infected juvenile kittens. These kittens either acquired infection by natural vertical transmission or were experimentally inoculated with the virus at defined times of fetal or neonatal life. Thymocytes from FIV-infected cats were analyzed by flow cytometry for the differential expression of CD4, CD8, Pan T, and IgG and subpopulation percentages were compared to values from uninfected littermates. Infected cats demonstrated a decrease in the percentage of CD4+/CD8+ lymphocytes and a concurrent increase in the percentage of CD4-/CD8-, CD4-/CD8+, and IgG+ lymphocytes. Absolute numbers of IgG+ cells were increased with FIV infection. On bivariate distribution scatter plots generated by two-color flow cytometry, this population of IgG+ cells overlapped extensively with cells having low to minimally detectable levels of a pan-T lymphocyte marker, suggesting that thymocytes were coated with IgG. Immunohistochemical detection of feline IgG defined a broad zone of IgG+ cells within the residual cortex but outside lymphoid follicles. However, cells stained with B5, a feline B lymphocyte marker, localized almost exclusively to the centers of lymphoid follicles that were also characterized by a lack of internal cytokeratin staining. FIV RNA transcripts detected by in situ hybridization using an FIVgag RNA probe were evenly distributed throughout the thymic parenchyma except in lymphoid follicles, which were generally devoid of FIV expression. Despite these phenotypic and structural changes, thymus weight, expressed as a percentage of body weight, was not significantly reduced. From these data, we conclude that the clinically asymptomatic stage of FIV infection is associated with two distinct B cell-related phenomena within the thymus-the formation of germinal centers and the coating of thymocytes with IgG. These changes accompany a distorted thymocyte distribution characterized by a reduced percentage of CD4+/CD8+ lymphocytes and a relative increase in CD4-/CD8+ and CD4-/CD8- lymphocytes. Together, these findings suggest that degenerative thymic changes after lentivirus infection may involve humoral immune mechanisms.
通过检测感染猫免疫缺陷病毒(FIV,一种艾滋病动物模型)的幼年小猫胸腺细胞的表型组成、胸腺上皮细胞结构以及胸腺中病毒RNA的转录,对胸腺改变进行了研究。这些小猫要么通过自然垂直传播获得感染,要么在胎儿期或新生儿期的特定时间通过实验接种该病毒。通过流式细胞术分析FIV感染猫的胸腺细胞,以检测CD4、CD8、泛T细胞和IgG的差异表达,并将亚群百分比与未感染同窝小猫的值进行比较。感染猫的CD4+/CD8+淋巴细胞百分比降低,同时CD4-/CD8-、CD4-/CD8+和IgG+淋巴细胞百分比增加。FIV感染使IgG+细胞的绝对数量增加。在双色流式细胞术生成的双变量分布散点图上,这群IgG+细胞与泛T淋巴细胞标志物水平低至几乎检测不到的细胞广泛重叠,表明胸腺细胞被IgG包被。猫IgG的免疫组织化学检测在残留皮质内但在淋巴滤泡外定义了一个广泛的IgG+细胞区。然而,用猫B淋巴细胞标志物B5染色的细胞几乎只定位于淋巴滤泡中心,这些中心的特征也是缺乏内部细胞角蛋白染色。使用FIVgag RNA探针通过原位杂交检测到的FIV RNA转录本均匀分布在整个胸腺实质中,但淋巴滤泡中通常没有FIV表达。尽管有这些表型和结构变化,但以体重百分比表示的胸腺重量并未显著降低。根据这些数据,我们得出结论,FIV感染的临床无症状阶段与胸腺内两种不同的B细胞相关现象有关——生发中心的形成和胸腺细胞被IgG包被。这些变化伴随着胸腺细胞分布的扭曲,其特征是CD4+/CD8+淋巴细胞百分比降低,CD4-/CD8+和CD4-/CD8-淋巴细胞相对增加。总之,这些发现表明慢病毒感染后的胸腺退行性变化可能涉及体液免疫机制。
