Cullen Cheryl L, Wadowska Dorota W, Singh Amreek, Melekhovets Yuri
Department of Companion Animals, Atlantic Veterinary College, University of Prince Edward Island, 550 University Avenue, Charlottetown, Prince Edward Island, Canada.
Vet Ophthalmol. 2005 Sep-Oct;8(5):295-303. doi: 10.1111/j.1463-5224.2005.00402.x.
(1) To describe the ultrastructural features of corneal sequestra in cats; and (2) to enhance our understanding regarding the pathogenesis of feline corneal sequestration.
Nine corneal sequestra were harvested via keratectomy from globes of nine cats. The sequestra were routinely fixed then postfixed for high resolution light and transmission electron microscopy (HR-LM and TEM, respectively). The tissues were embedded in Epon/Araldite. Sections of 0.5-microm thickness were cut and stained with 1% toluidine blue in 1% sodium tetraborate solution for HR-LM. Ultrathin sections were collected on copper grids and stained with uranyl acetate and Sato's lead stain for TEM. Ultrathin sections were examined and the images were captured on an Advantage HR CCD camera using a Hitachi 7500 electron microscope operated at 80 kV. Two healthy corneas from two cats were harvested immediately following euthanasia. These corneal tissues (control samples) were processed in the same manner as the corneal sequestra for HR-LM and TEM. A portion of each sequestrum was also submitted for polymerase chain reaction (PCR) testing for infectious agents including feline herpesvirus-1 (FHV-1), Toxoplasma gondii, Chlamydophila felis and Mycoplasma spp.
Ultrastructure of healthy corneal tissues revealed basal corneal epithelial cells aligned adjacent to a thin acellular layer similar to Bowman's layer with underlying tightly packed, regularly arranged, collagen fibrils oriented in different planes. Keratocytes were elongated and had long and irregularly shaped nuclei, and cytoplasm contained rough endoplasmic reticulum and abundant membrane-bound vesicles. In contrast, corneal sequestra contained varying amounts of an amorphous, electron-dense substance, continuous with intact basal epithelial basement membranes peripherally, and overlying corneal ulceration and loosely packed collagen fibrils. Remnants of necrotic keratocytes were seen in spaces between disarranged collagen layers. In all samples, occasional keratocytes exhibited morphology indicative of apoptosis including clumping and margination of chromatin, and shrunken cytoplasm. Varying degrees of inflammation were noted on HR-LM and TEM of affected corneas including peri- and intralesional neutrophils, lymphocytes, plasma cells, and macrophages. Corneal sequestra were FHV-1-positive (n = 3), FHV-1- and T. gondii-positive (n = 1), T. gondii-positive (n = 3), or negative for DNA of these infectious agents (n = 2) using PCR. All corneal sequestra were negative for DNA of Chlamydophila felis and Mycoplasma spp. using PCR.
Apoptosis may play a role in the pathogenesis of feline corneal sequestration independent of the presence of DNA of these infectious organisms. Prospective clinical studies are warranted to further understand the significance of T. gondii in relation to feline corneal sequestration.
(1)描述猫角膜腐骨的超微结构特征;(2)加深我们对猫角膜腐骨发病机制的理解。
通过角膜切除术从9只猫的眼球中获取9个角膜腐骨。将腐骨常规固定,然后进行后固定,分别用于高分辨率光学显微镜和透射电子显微镜检查(分别为HR-LM和TEM)。组织包埋于环氧树脂/阿拉底胶中。切取0.5微米厚的切片,用1%四硼酸钠溶液中的1%甲苯胺蓝染色用于HR-LM。超薄切片收集在铜网上,用醋酸铀和佐藤铅染液染色用于TEM。检查超薄切片,并使用在80 kV下操作的日立7500电子显微镜在Advantage HR CCD相机上采集图像。在安乐死后立即从2只猫获取2个健康角膜。这些角膜组织(对照样本)按照与角膜腐骨相同的方式进行处理,用于HR-LM和TEM。每个腐骨的一部分还进行聚合酶链反应(PCR)检测,以检测包括猫疱疹病毒-1(FHV-1)、弓形虫、猫衣原体和支原体属在内的感染因子。
健康角膜组织的超微结构显示,基底角膜上皮细胞与一层类似于Bowman层的薄无细胞层相邻排列,其下方紧密堆积、规则排列的胶原纤维在不同平面上定向排列。角膜细胞呈细长形,具有长且形状不规则的细胞核,细胞质中含有粗面内质网和丰富的膜结合小泡。相比之下,角膜腐骨含有不同数量的无定形、电子致密物质,其周边与完整的基底上皮基底膜连续,覆盖角膜溃疡和松散堆积的胶原纤维。在排列紊乱的胶原层之间的间隙中可见坏死角膜细胞的残余物。在所有样本中,偶尔可见角膜细胞呈现凋亡形态,包括染色质凝聚和边缘化以及细胞质收缩。在受影响角膜的HR-LM和TEM检查中发现不同程度的炎症,包括病灶周围和病灶内的中性粒细胞、淋巴细胞、浆细胞和巨噬细胞。使用PCR检测,角膜腐骨FHV-1阳性(n = 3)、FHV-1和弓形虫阳性(n = 1)、弓形虫阳性(n = 3)或这些感染因子的DNA阴性(n = 2)。所有角膜腐骨使用PCR检测猫衣原体和支原体属的DNA均为阴性。
凋亡可能在猫角膜腐骨的发病机制中起作用,与这些感染性生物体DNA的存在无关。有必要进行前瞻性临床研究,以进一步了解弓形虫与猫角膜腐骨的关系。
Zotero 插件