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利用荧光显微镜和电子显微镜对发育中的鹦鹉热衣原体包涵体进行时间分析。

Temporal analysis of the developing Chlamydia psittaci inclusion by use of fluorescence and electron microscopy.

作者信息

Rockey D D, Fischer E R, Hackstadt T

机构信息

Rocky Mountain Laboratories, National Institute of Allergy and Infectious Diseases, Hamilton, Montana 59840, USA.

出版信息

Infect Immun. 1996 Oct;64(10):4269-78. doi: 10.1128/iai.64.10.4269-4278.1996.

Abstract

The chlamydiae are obligate intracellular parasites that develop and multiply within a vacuole (termed an inclusion) that does not fuse with lysosomes. Inclusion morphology varies dramatically among the different chlamydiae, particularly within the species Chlamydia psittaci. Some strains develop within a single vacuole, while the mature inclusion of other strains consists of several distinct lobes, each filled with chlamydial developmental forms. The development of this lobed structure was investigated in HeLa cells infected with the guinea pig inclusion conjunctivitis (GPIC) strain of C. psittaci. We employed two recently described probes for the chlamydial inclusion to study the development of these unique lobed structures. The novel probes were an antiserum directed at a protein localized to the GPIC inclusion membrane (anti-IncA) and the fluorescent sphingolipid (N-[7-(4-nitrobenzo-2-oxa-1,3-)]) aminocaproyl sphingosine (NBD-ceramide). Lobed inclusions developed in cells infected at very low multiplicities of infection, suggesting that the structure is not a function of infection by more than one elementary body (EB). Double-label fluorescent-antibody analysis with anti-IncA and an antibody directed at a chlamydial outer membrane protein showed that, prior to 18 h postinfection (p.i.), the inclusion membrane and the chlamydial membrane were tightly associated. After 18 to 20 h p.i., the lobes began to expand and fill with developmental forms and the inclusion membrane and chlamydial membrane became distinct. At times from 8 to 48 h p.i., GPIC inclusions were shown to receive fluorescent derivatives of NBD-ceramide and to be localized to the perinuclear region of the host cell. Labeled lectins with affinity for carbohydrate moieties localized to the Golgi apparatus showed that the lobes of mature inclusions surround the Golgi apparatus. Labeling with NBD-ceramide and the Golgi apparatus-specific lectins therefore demonstrated a functional and physical association of the inclusion with the Golgi apparatus throughout the developmental cycle. Collectively, these results lead to a model for the development of the lobed chlamydial inclusion. We propose that the lobed structure is a result of division of inclusions occurring in parallel with the multiplication of reticulate bodies (RB) early in the developmental cycle. The division of inclusions slows or stops in mid-cycle, and dividing RB accumulate within the enlarging lobes. The RB then differentiate to EBs, the inclusion and cell are lysed, and EBs are freed to infect another cell.

摘要

衣原体是专性细胞内寄生虫,在不与溶酶体融合的液泡(称为包涵体)内发育和繁殖。不同衣原体的包涵体形态差异很大,尤其是鹦鹉热衣原体种内。一些菌株在单个液泡内发育,而其他菌株的成熟包涵体由几个不同的叶组成,每个叶都充满衣原体发育形式。在感染鹦鹉热衣原体豚鼠包涵体结膜炎(GPIC)菌株的HeLa细胞中研究了这种叶状结构的发育。我们使用了两种最近描述的针对衣原体包涵体的探针来研究这些独特叶状结构的发育。这两种新型探针分别是针对定位于GPIC包涵体膜的一种蛋白质的抗血清(抗-IncA)和荧光鞘脂(N-[7-(4-硝基苯并-2-恶唑-1,3-)]氨基己酰鞘氨醇(NBD-神经酰胺)。在感染复数非常低的细胞中形成了叶状包涵体,这表明该结构不是由多个原体(EB)感染的结果。用抗-IncA和针对衣原体外膜蛋白的抗体进行的双标记荧光抗体分析表明,在感染后(p.i.)18小时之前,包涵体膜和衣原体膜紧密相连。在感染后18至20小时,叶开始扩展并充满发育形式,包涵体膜和衣原体膜变得明显分开。在感染后8至48小时的各个时间点,GPIC包涵体被证明摄取了NBD-神经酰胺的荧光衍生物,并定位于宿主细胞的核周区域。对定位于高尔基体的具有对碳水化合物部分亲和力的标记凝集素显示,成熟包涵体的叶围绕着高尔基体。因此,用NBD-神经酰胺和高尔基体特异性凝集素进行标记证明了在整个发育周期中包涵体与高尔基体之间存在功能和物理联系。总的来说,这些结果得出了一个叶状衣原体包涵体发育的模型。我们提出叶状结构是发育周期早期与网状体(RB)增殖同时发生的包涵体分裂的结果。包涵体的分裂在周期中期减缓或停止,分裂的RB聚集在扩大的叶内。然后RB分化为EB,包涵体和细胞裂解,EB释放出来感染另一个细胞。

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