白色念珠菌对上皮细胞粘附性的观察

念珠菌性口腔炎是口腔的常见疾病 ,病原体以白色念珠菌多见。据报道 [1、2 ] ,口腔粘膜上皮细胞对念珠菌的粘附性与上皮细胞的分化程度有关。我们从健康人的口腔粘膜获取上皮细胞标本 ,与白色念珠菌混合孵育后 ,应用巴氏染色方法来观察念珠菌对各类上皮细胞的粘附性能。1　材料与方法1.1　粘膜上皮细胞的制备　选择 2 0例健康人 (男性 10名 ,女性 10名 ,年龄 30～ 4 0岁 ) ,用无菌棉拭子在口腔粘膜表面反复轻擦 ,将棉试子浸入无菌磷酸盐缓冲液内 (PBS;0、0 1mol/ L ,p H7、2 ) ,摇动棉拭子使上皮细胞落于 PBS中 ,细胞悬液离心 15 min(10…     

白色念珠菌粘附口腔粘膜上皮细胞配体的初步研究

目的：研究白色念珠菌对口腔粘膜上皮细胞的粘附配体,方法：采用体外法测定白色念珠菌对口腔上皮细胞的粘附数量,结果：D－甘露糖预作用于上皮细胞之后,可以使白色念珠菌粘附下降,刀豆素A及绿慕安预作用于白色念珠菌,可以减少白色念珠菌对上皮细胞的粘附,结论：白鬼念珠菌粘附感染与其表面甘露糖结构有关。     

白色念珠菌和热带念珠菌对人肺上皮细胞的粘附作用及其差异性比较

目的探讨白色念珠菌和热带念珠菌对人肺上皮细胞的粘附作用及其差异性.方法将白色念珠菌和热带念珠菌临床分离株在体外与人肺上皮细胞共同作用,经革兰染色后,在倒置显微镜下观察念珠菌对肺上皮细胞的粘附数.结果念珠菌粘附的肺上皮细胞与浓度和时间有依赖关系.菌液浓度在5×103CFU/ml至5×107CFU/ml范围内,念珠菌对肺上皮细胞的粘附作用随念珠菌浓度的增加而增强.白色念珠菌对肺上皮细胞的粘附数比热带念珠菌的粘附数要高.来自痰、尿标本的同一种念珠菌对人肺上皮细胞的粘附数无明显差异.结论念珠菌对人肺上皮细胞的粘附是一种特异性的粘附,临床标本来源的白色念珠菌粘附宿主细胞的能力比热带念珠菌强.     

阻断白色念珠菌粘附口腔膜上皮细胞的实验研究

白色念珠菌的粘附与其表面甘露糖结构有关,为探讨阻断粘附的方法,我们采用体外法测定其对口腔上皮细胞的粘附数量,显示：白色念珠菌粘附感染上皮细胞后,甘露糖可以在一定程度上减少粘附,绿慕安及刀豆素A可以有效地减少粘附。提示甘露糖及绿慕安可能有助于治疗白色念珠菌感染。     

白色念珠菌粘附的研究进展

本文论述了白色念珠菌（简称白念菌）粘附的分子机理和实验模型观察,从病原菌和宿主两方面探讨了白念菌感染的发病机理,并从阻断白念菌对宿主细胞的粘附着手,展望防治白念菌感染的新途径和措施。     

白念珠菌粘附上皮细胞的机制

本文总结了近年来白念珠菌细胞表面疏水性、侵袭性酶、以及表面甘露糖、蛋白质等对上皮细胞粘附的研究进展,提出了阻断白念珠菌粘附的方式。     

肉桂醛对根管内白色念珠菌生物膜作用的体外研究

目的研究肉桂醛对体外白色念珠菌生物膜的影响。方法采用琼脂扩散法进行肉桂醛和洗必泰对白色念珠菌敏感性的比较;MTT法评价肉桂醛对白色念珠菌生物膜及细胞黏附的影响。结果 2 048μg/mL肉桂醛与2%洗必泰抑菌环直径比较差异无统计学意义(P>0.05);4 096μg/mL肉桂醛对白色念珠菌生物膜的抑菌率达93.02%;不同浓度肉桂醛对60、90和120 min的白色念珠菌细胞粘附都具有抑制作用。结论肉桂醛对体外白色念珠菌生物膜有较明显的抑制作用。     

白色念珠菌蛋白酶与其毒力关系的研究

目的 探讨白色念珠菌蛋白酶活动与其毒力关系。方法的采用牛奶平地检测５４株白色念珠菌蛋白酶的分泌能力,然后选择６侏菌分别经摇瓶培养测定其蛋白酶活力,并以静脉内注射方式感染小鼠进行毒力试验,以小鼠平均生存时间来评价菌株毒力。结果 ５４株白色念珠菌全部能分泌蛋白酶,检出率为１００％。动物试验表明蛋白酶活力愈高的菌株,相应小鼠平均生存时间愈短;蛋白酶活力与菌株毒力直接正相关（γ＝０．９３４,Ｐ＜０．０１）     

钛合金和钴铬合金表面白色念珠菌粘附的研究

目的比较钛合金(Ti-6Al-4V)和钴铬合金(Chromium-Cobaltalloy)表面白色念珠菌粘附能力的大小,研究表面粗糙度与细菌粘附的关系。方法将不同表面粗糙度的钛合金和钴铬合金试件进行白色念珠菌体外粘附试验,采用菌落形成计数法测定试件表面的细菌粘附量。结果各钛合金试件组的细菌粘附量均少于相同表面粗糙度的钴铬合金试件组,两种金属试件表面的细菌粘附量均随表面粗糙度的增大而增加。结论钛合金较钴铬合金更能减少由白色念珠菌引起的义齿性口炎等并发症,同时修复体表面严格的研磨抛光也能有效减少这些并发症。     

Adherence of Candida albicans to host cells

Abstract Research devoted to uncovering the mechanisms of adherence of Candida albicans to human tissue is reviewed. The physical aspects of adherence of the fungus to host cells and the biochemical and molecular features, as far as they are known, are discussed. Relevant pre- and post-adherence events in the pathogenesis of disease caused by this fungus are also noted. Putative adhesins and surface receptors of C. albicans for host proteins are discussed in detail.     

Adherence of germ tubes of Candida albicans to tissues from immunocompromised mice

Abstract The influence of immune status of the host on binding of germ tubes of Candida albicans to murine tissue sections in an ex vivo assay was examined. Generally, germ tubes appeared randomly adhered to the tissues examined and binding was unaffected by immunodeficiency induced by treatment with cyclophosphamide and cortisone acetate. Adherence was somewhat reduced in spleen and kidney sections or increased in liver sections and unchanged in lymph node sections from treated mice compared to sections from control animals. Scanning electron micrographs showed organisms appeared to be loosely or tightly bound to the surface or partially embedded in spleen sections from both control and treated mice. These observations suggested that qualitative and quantitative difference in adhesion of germ tubes to various tissues may contribute little to the susceptibility of the immunodeficient animal to candidal infection.     

Infection of HEp2 epithelial cells with Candida albicans: adherence and postadherence events

We have previously observed that the infection of HEp2 epithelial cells with Candida albicans results in HEp2 cell actin rearrangement, and that a culture filtrate of C. albicans (Candida metabolite) caused the same changes and reduced membrane ruffling and motility. It was found that the Candida metabolite consisted of several proteins and nonproteinaceous components. In this study we report on the identity of three of the main proteins in the Candida metabolite, namely a secretory aspartate protease (Sap), an agglutinin-like adhesion sequence (Als) and a glucan 1,3-beta-glucosidase. The effect on HEp2 cells caused by the Candida metabolite, an inhibitor of the PKC MAP kinase signal pathway - bisindolylmaleimide (BIM), or the actin polymerization inhibitor - cytochalasin D (CyD) were studied alone and in combination. Exposure of HEp2 cells to the Candida metabolite, together with the BIM or CyD, had profound effects on HEp2 cell morphology, as compared to individually treated cells, and also reduced the adherence of the organisms to HEp2 cells. Our results show that the interaction of C. albicans with HEp2 cells is, not unexpectedly, complex, and involves changes in the host cell that may be related to the effect of Candida-secreted biomolecules.     

紫外线对白念珠菌的影响

紫外线作为重要的环境因子之一,能显著影响包括白念珠菌在内的多种生物的生长及生理过程.研究发现白念珠菌受紫外线照射后菌丝形成被抑制,孢子形成增多且没有向光性;脉冲紫外线辐射可通过多靶点程序使白念珠菌失活;rad 51缺陷株比rad 52缺陷株更易受紫外线损害,同时紫外线可导致白念珠菌杂合性丢失.研究还发现UVC治疗可明显减少烧伤后真菌微生物感染,核黄素/UVA治疗可明显抑制白念珠菌生长.因此紫外线对白念珠菌有一定的抑制作用.     

定菌生调整实验小鼠念珠菌性阴道炎的菌群失调的研究

目的 应用阴道细菌培养与光镜细胞学检查相结合的方法,研究定菌生对阴道念珠菌感染的菌群失调的调整作用。方法 以小鼠为实验对象,用盐酸林可霉素造成阴道菌群失调,并将分离的念珠菌接种到小鼠阴道内,造成小鼠阴道念珠菌感染模型,分别采用定菌生、抗真菌＋定菌生及抗真菌（制霉菌素）治疗1疗程后,取其阴道分泌物进行念珠菌及乳杆菌的菌群分析,并同时进行分泌物镜检,取阴道组织标本做病理组织学检查。结果 模型组小鼠阴道内主要细菌数量乳杆菌显著下降（P〈0．01）．出现阴道红肿、分泌物多呈块状和阴道黏膜充血等念珠菌阴道炎的典型症状,分泌物涂片镜检查到白细胞及念珠菌,而定菌生组和定菌生＋制霉菌素组治疗的小鼠,阴道黏膜与健康对照组的阴道黏膜基本相同,阴道内主要菌群——乳杆菌的数量恢复正常,阴道内念珠菌显著降低,与自然恢复组相比差异有极显著性（P〈0．01）,与制霉菌素处理比差异也有显著性,治疗效果明显好于制霉菌素。结论 定菌生能阻止念珠菌对阴道上皮的粘附作用,能调整阴道的菌群,对阴道黏膜有一定的修复功能,是治疗念珠菌性阴道炎有效的微生态调节剂。     

Adherence of Candida species to fibrin clots in vitro

The adherence of six Candida species to fibrin clots was studied using a simple, in vitro technique. Yeast suspensions were incubated with fibrin clots and the number of adherent organisms quantified as follows: after washing, the clots were subjected to vortex mixing and the number of CPU's which subsequently grew on Sabourauds medium were counted. Adhesion was directly proportional to the concentration of Candida species in the suspension (r=0.99 p<0.001). C. albicans and C. tropicalis exhibited marked adherence whereas C. krusei, C. gulliermondi and C. glabrata adhered less readily. C. parapsilosis was intermediate in its ability to adhere.     

Adhesion of Candida albicans mutant strains to host tissue

Adhesion of Candida albicans to host cells is believed to represent a fungal virulence factor and a significant step in the development of candidiasis. As C. albicans strains may differ in their in vitro adhesion ability we initiated a study to investigate whether mutant strains differ in this respect from their parent wild-type. We assessed the in vitro adhesion of C. albicans CBS562 and two mutants obtained by mutagenesis with N′-nitrosoguanidine: a histidine auxotroph, SAG5, derived from CBS562, and a respiratory-deficient strain (a petite mutant), SAR1, derived from SAG5. The adhesion was tested in vitro using two target cell systems: (1) exfoliated human buccal epithelial cells (BEC); and (2) human keratinocyte tissue line cells (HaCaT cells). Adhesion to BEC was evaluated microscopically and that to HaCaT cells by a direct ELISA technique. The results indicated a 54% reduction in adhesion to BEC for SAG5 and 30% for SAR1 as compared to the wild-type, and a 25% reduction in adhesion to HaCaT cells for SAG5 and 20% for SAR1. To verify whether the prototrophy restores the adhesion ability, we complemented the his-negative auxotroph by transforming the strain with the HIS4 gene. Then we assayed the adhesion to BEC of the complemented his-negative mutant in comparison to that of the wild-type, the his-negative mutant (SAG5) and the plasmid-cured transformant. The adhesion values of the complemented his-negative strain were similar to those of the wild-type, whereas the values of the plasmid-cured strain were similar to those of SAG5.     

白念珠菌破壁方法的研究应用进展

细胞壁作为真菌中特殊和必须的细胞结构,相对于哺乳动物的细胞膜更加坚硬,难以用简单的方法使其充分破碎。因此,达到理想的破壁效果是白念珠菌研究中的关键步骤之一。在提取白念珠菌RNA、DNA和蛋白质等细胞组分的过程中,为获得足量和稳定的实验样品。该文对多种白念珠菌破壁方法作一综述,以便为白念珠菌相关研究提供适用、高效的破壁方案。     

都柏林念珠菌的鉴定及与白念珠菌3种表型鉴别方法的研究

目的 从临床分离的念珠菌中进一步鉴定都柏林念珠菌,并评价3种表型鉴别白念珠菌和都柏林念珠菌的方法.方法 对17株临床分离并初步鉴定的白念珠菌和1株ATCC白念珠菌标准株,采用PHR1同源序列PCR法检测,鉴定出其中的都柏林念珠菌;分别采用45℃生长试验、YEPD(1%酵母浸膏,2%蛋白胨,2%葡萄糖)液基39℃芽管生成试验、Staib琼脂(鸟食琼脂)厚壁孢子形成试验对两种菌的表型特点进行比较.结果 17株临床分离的白念珠菌中有3株鉴定为都柏林念珠菌;45℃时,两种菌在改良沙堡弱琼脂上均无明显生长,YEPD液基中仅有1株白念珠菌生长良好;YEPD液基39℃培养2种菌均无芽管生成;Staib琼脂培养72h,3株都柏林念珠菌中有2株可形成厚壁孢子,而白念珠菌则无,与PHR1同源序列检测结果基本一致.结论 PHR1同源序列检测是鉴别都柏林念珠菌与白念珠菌的可靠方法,Staib琼脂厚壁孢子形成试验有助于鉴别两菌,45℃生长试验和YEPD液基39℃芽管生成试验则不能有效鉴别两菌.