川金丝猴柯萨奇病毒的分离鉴定

利用细胞培养方法从长春某动物园送检的死亡川金丝猴心脏中分离获得1株柯萨奇病毒,经系统的形态学、理化学、动物回归试验和RT-PCR扩增,符合柯萨奇B型病毒特征;进而对其VP1基因部分序列和特异性血清抗体分析,证明所分离的病毒为柯萨奇B3型病毒.这是国内外首次从金丝猴分离到该病毒,暂命名为CVB/SGM-05.     

绵羊肺源性致病性大肠杆菌的分离与鉴定

【目的】近年来,羊呼吸系统疾病日益频发,由肠外致病性大肠杆菌感染引起的呼吸道疾病也日渐增多,给养羊业带来了一定经济损失。本文旨在确定新疆石河子地区某羊场表现为呼吸道感染症状的病死羔羊的细菌性病原及其特性。【方法】采用细菌常规分离鉴定结合16S rRNA基因序列分析的方法从发病羔羊的肺脏中分离鉴定细菌,并对分离株进行药敏试验、特异基因PCR检测、小鼠致病性试验及肺脏组织的病理学观察。【结果】从病死羔羊肺脏组织分离得到一株致病性大肠杆菌,该分离株呈多重耐药现象,检测到iutA、fyuA和ireA三种毒力基因;病变肺脏肺泡壁毛细血管充血,界限不清,支气管管腔充血,周围淋巴细胞浸润、增生。【结论】从病死羔羊肺中分离的细菌性病原是肠外致病性大肠杆菌(ExPEC)。     

裸鼠巴斯德氏菌病的诊断

目的对某实验动物中心裸鼠发病死亡的原因进行诊断。方法对发病裸鼠进行病理组织学和细菌学检查以及血清学试验。结果根据临床症状、病理剖检、细菌分离培养、生化鉴定和血清凝集试验,确诊为嗜肺巴斯德氏菌感染导致的细菌性疾病。药敏试验结果表明,分离菌株对阿莫西林／克拉维酸、阿奇霉素、复方新诺明敏感,而对红霉素已经产生耐药性。结论为巴斯德氏菌病原鉴定与疾病诊断提供了科学依据。     

非典型肺炎病例标本中新型冠状病毒的分离与鉴定

目的对非典型肺炎的病原体进行分离鉴定,为该病的诊断、预防和治疗提供依据。方法采用细胞培养和乳鼠接种法,从非典型肺炎病例标本中分离致病病原体,通过电镜形态学、血清学和动物致病性观察及RTPCR扩增与部分基因序列分析,对分离的病原体进行鉴定。结果成功地从死亡病例尸解的肺组织标本和患者鼻咽拭子标本中采用细胞培养法分离出病原体。通过电镜在病变细胞及其培养上清中观察到大量冠状病毒样颗粒。免疫荧光染色检测非典型肺炎患者血清,表明分离的病毒与此次流行的非典型肺炎密切相关。分离的病毒可对乳鼠致病,并在发病乳鼠的肺组织标本中通过电镜同样观察到冠状病毒样颗粒。从非典型肺炎病例尸解肺组织、传代发病小鼠肺组织及分离物感染的细胞培养物中,通过RTPCR可分别扩增出冠状病毒的cDNA片段,测序结果显示其核苷酸序列与已知冠状病毒的同源性在60%左右。结论从非典型肺炎病例标本中已成功分离出一种新的冠状病毒,它与此次流行的非典型肺炎密切相关,很可能是此次流行的非典型肺炎的主要病原体 。     

松鼠猴感染假结核耶尔森菌的诊治

2013 年2 月18 - 20 日,四川省雅安市碧峰峡野生动物园内6 只松鼠猴突然接连死亡,同时约有100 只松鼠猴也出现了不同症状,给动物园造成了严重的损失。为寻找传染病因和治疗防控措施,首先采用尸体剖解和病理切片对其进行了组织学检查,然后采用细菌分离培养和鉴定确定了病原菌,通过动物回归试验和耐药性试验发现其致病性和流行性特征,并采取紧急治疗和防疫措施及时控制了疫情。结果表明,死猴尸体内多处器官发生淤血坏死,组织病变严重并可见大量细菌。经鉴定,分离到的病原细菌为假结核耶尔森菌,该菌与鼠疫耶尔森菌同源性极高,且具有强烈的致病性、传染性和一定的耐药性,对丁胺卡拉霉素较为敏感。这是我国首次发现并报道的松鼠猴感染假结核耶尔森菌病例,本文对其诊断与治疗、流行病学研究和病理模型建立提供了一定的基础参考资料。     

云南森林脑炎病毒的动物敏感性研究

本文对分离自云南的森林脑炎病毒进行了动物敏感性研究,实验证明云南森林脑炎病毒对小白鼠有较强的致病性,三日龄乳鼠无论经脑内、腹腔、皮下接种均能致病、死亡,但毒力较国内森林脑炎病毒标准株低;三周龄小白鼠经鼻腔接种亦能发病致死。对乳大白鼠、幼年豚鼠和金黄色地鼠能引起发病或死亡,病毒抗原定位主要在脑组织。病理检查表明感染的各种动物脑组织均有明显病变。此外,对鸡胚敏感,能引起BHK_(21)、Vero、Vero-E_6等传代细胞及人胚肾、乳猪肾原代细胞的CPE_0结果表明了云南森林脑炎病毒对细胞、动物的致病性与国内森林脑炎病毒标准株相似,仅毒力稍低。     

流行性乙型脑炎强毒株和弱毒疫苗株SA14-14-2对猴子和小鼠的致病性和病理学研究

为了解乙型脑炎 (乙脑 )减毒活疫苗弱毒株SA14 14 2神经毒力的减弱程度 ,本文对弱毒株及其原株SA14强毒株进行了猴体和小白鼠的致病性和病理学变化的比较试验。SA14强毒株病毒 (原始滴度 6 15× 10 8/ml) ,以10 -2 和 10 -4 ～ 10 -7不同稀释度于丘脑两侧合并脊髓注射恒河猴 ,每组除 10 -4 1只外其余均为 2只。另以 10 -4 和10 -6～ 10 -8不同稀释度脑内注射小鼠 ,每组 8只。结果猴子除 10 -4 1只外其余全部发病死亡 ,小鼠则全部死亡。SA14 14 2以 1∶5稀释病毒 (原始滴度为 8× 10 6/ml)按同样方法注射 4只猴和 30只小鼠 ,结果全部存活。另以SA1410 -2 病毒皮下注射 3只猴未死亡 ,而以 10 -1皮下注射 30只小鼠时则全部死亡。SA14 14 2以 1∶5稀释病毒皮下注射小鼠时则全部存活。病理组织学结果显示二种动物接种SA14株强毒后主要表现为弥散性脑脊髓炎 ,以神经细胞坏死为其主要特征和最突出的病变。猴子的病变以脊髓前角、丘脑和中脑黑质为重 ,小鼠的病变则以大脑皮质、海马部最重 ,脊髓的病变却比脑轻。接种弱毒株的动物则仅有轻微炎症反应、神经细胞坏死极少出现。以上结果表明以脑内接种时恒河猴和小鼠对乙脑病毒均高度敏感 ,以皮下接种时小鼠的敏感性高于猴子。乙脑SA14 14 2弱毒株的神经毒力包括致     

雏鸡源致病性粪肠球菌的分离鉴定及其耐药性分析

【背景】粪肠球菌(Enterococcus faecalis)是人和动物肠道正常菌群之一,也是一种条件性致病菌。近年来,粪肠球菌引起人和动物感染的报道越来越多。【目的】探明引起某养鸡场雏鸡发病死亡的病原及其致病性和有效治疗药物。【方法】结合临床症状和病理剖检,开展病原菌分离、生理生化特性检测和16S rRNA基因序列分析、致病性试验、耐药分析和对患病鸡群的药物治疗。【结果】患病鸡有昏睡、瘫痪或共济失调等临床症状;肝、脾肿大,肝脏发黄、少量出血点、质脆易碎,肠道粘膜增厚、出血,脑轻微水肿;从肝脏组织分离得到一株革兰氏阳性球菌,经纯化培养后命名为CJ517;依据该菌株形态特征、生理生化特性和16S rRNA基因序列分析鉴定为粪肠球菌;致病性试验显示CJ517菌株能致死小鼠,致死率为66.67%;该菌对头孢噻肟、磷霉素、丁胺卡那等药物敏感,对多西环素、卡那霉素、新霉素、氟苯尼考等药物耐药;经用敏感药物和提高免疫力结合治疗后,鸡群病情得到控制。【结论】研究结果可为临床诊断和治疗动物粪肠球菌感染提供参考。     

宿主特异性差异导致沙门氏菌在猪体内定植对特定基因要求的不同

自1885年Salmon等分离得到猪霍乱沙门氏菌以来,目前已检出沙门氏菌血清型2 500余种。沙门氏菌(salmonella)属的成员可感染多种动物和人,大部分具有很强的致病性。其中许多血清型菌能在人和动物之间交叉感染。目前,人们利用全身性疾病小鼠模型对沙门氏菌的致病性做了大量的研究。常用的小鼠模型与体外细胞培养分析相结合,这一     

禽流感H5N1亚型病毒对五个不同品系小鼠致病性的比较(英文)

目的比较了不同遗传背景小鼠对禽流感H5N1亚型病毒的致病敏感性,为H5N1禽流感模型制作和机理研究提供依据。方法近交系BALB/c、C57BL/6和封闭群ICR、NIHSwiss和KMSwiss共五个不同品系小鼠。每个品系实验动物30只,分接毒组20只,空白对照组10只,每组雌雄各半。病毒株为A/Goose/Guangdong/NH/2003(H5N1),经测定TCID50为10-4.875/mL。接毒组通过鼻腔接种0.1mL病毒液,对照组接种正常鸡胚尿囊液。小鼠接毒后连续观察14d,观察记录临床症状、体温、体重变化,对在实验期间死亡和实验14d结束后仍然存活的小鼠均进行组织器官病理取材,进行RT-PCR病毒分离检测、HE染色及H5N1抗原特异性免疫组化染色。结果①临床症状:H5N1禽流感病毒能感染五个品系的小鼠,引起呼吸急促等症状和一过性体重、体温下降。②死亡情况:小鼠在接毒后第1天即出现死亡,死亡的高峰期集中在接毒后第3～6天。五个品系小鼠死亡率存在差异,BALB/c为70%,ICR为50%,NIHSwiss为40%,C57BL/6为25%,KMSwiss为10%;③病毒分离:各组接毒小鼠在死亡后均进行了病毒分离,死亡小鼠的肺脏均分离到病毒,其他脏器未分离到病毒。④病理变化:实验期间五个品系死亡小鼠肺脏病理改变相近。大体观:死亡小鼠肺部淤血,呈暗红色,体积增大,局部肺组织实变。镜下观:死亡小鼠的共同病理改变为间质性肺炎,具体表现为肺泡腔及间质出血、炎性细胞浸润;间质增生,肺泡隔增宽;肺泡腔中见纤维素性渗出,透明膜形成。⑤免疫组化结果 :在死亡小鼠的气管上皮细胞和肺巨噬细胞可观察到H5N1禽流感病毒阳性表达。结论小鼠作为H5N1禽流感病毒模型具有普适性,不同品系小鼠感染鹅源H5N1禽流感病毒的临床症状、病程和病理变化与人禽流感病例相似。不同品系小鼠的死亡比例有明显差别,可以根据不同的实验目的 ,选择不同品系的小鼠制作H5N1禽流感动物模型。不同品系的遗传特性对禽流感易感性产生明显的影响,遗传背景可能与H5N1禽流感病毒感染应答机理存在联系:BALB/c和C57BL/6均为近交系,其中BALB/c小鼠的品系特征之一表现为干扰素产量低,接种H5N1病毒后表现为高死亡率(70%),而C57BL/6小鼠的干扰素产量高,接种H5N1病毒后表现为低死亡率(25%),提示不同遗传背景小鼠的干扰素水平与H5N1感染致死具相关性。为进一步研究H5N1禽流感病毒易感性相关基因以及其与宿主免疫反应的关系提供了一个研究基础。     

Complete Genome Sequence of a Coxsackievirus B3 Isolated from a Sichuan Snub-Nosed Monkey

Coxsackievirus B3 (CVB3) is an enterovirus in the family Picornaviridae that is significant to human health, being associated with myocarditis, aseptic meningitis, and pancreatitis, among other conditions. In addition to humans, Sichuan snub-nosed monkeys can be infected and killed by CVB3. Here, we report the first complete genome sequence of a novel coxsackievirus B3 strain, SSM-CVB3, which was isolated from a deceased Sichuan snub-nosed monkey with severe myocarditis. Our findings may aid in understanding the evolutionary characteristics and molecular pathogenesis of this virus.     

Autoantibodies specific for the cardiac myosin isoform are found in mice susceptible to Coxsackievirus B3-induced myocarditis

Several mouse strains are susceptible to immunopathic myocarditis after infection with Coxsackievirus B3 (CB3). This disease is associated with autoantibodies that are directed against myosin. In this study we characterized sera from CB3-infected mice for their reactivity with three different myosin isoforms (heart, skeletal muscle, and brain myosins) and for autoantibody isotype by using an ELISA. Competitive inhibition assays and absorption studies with various myosins demonstrated the presence of two autoantibody populations in sera of susceptible A.CA and A.SW mice. The first was specific for cardiac myosin and was mainly IgG. The second antibody population cross-reacted with heart, skeletal muscle, and brain myosin and was mainly IgM. B10.PL/SgSf and B10.A/SgSf mice, which do not develop immunopathic myocarditis, produced only the IgM autoantibody population cross-reactive with all three myosin isoforms. Because the heart-specific myosin autoantibodies were found exclusively in the mouse strains that developed immunopathic myocarditis, they can be considered a serologic marker for autoimmune heart disease.     

V gamma 1+ T cells suppress and V gamma 4+ T cells promote susceptibility to coxsackievirus B3-induced myocarditis in mice

Coxsackievirus B3 infections of C57BL/6 mice, which express the MHC class II IA but not IE Ag, results in virus replication in the heart but minimal myocarditis. In contrast, Bl.Tg.Ealpha mice, which are C57BL/6 mice transgenically induced to express IE Ag, develop significant myocarditis upon Coxsackievirus B3 infection. Despite this difference in inflammatory damage, cardiac virus titers are similar between C57BL/6 and Bl.Tg.Ealpha mice. Removing gammadelta T cells from either strain by genetic manipulation (gammadelta knockout(ko)) changes the disease phenotype. C57BL/6 gammadelta ko mice show increased myocarditis. In contrast, Bl.Tg.Ealpha gammadelta ko mice show decreased cardiac inflammation. Flow cytometry revealed a difference in the gammadelta cell subsets in the two strains, with Vgamma1 dominating in C57BL/6 mice, and Vgamma4 predominating Bl.Tg.Ealpha mice. This suggests that these two Vgamma-defined subsets might have different functions. To test this possibility, we used mAb injection to deplete each subset. Mice depleted of Vgamma1 cells showed enhanced myocarditis, whereas those depleted of Vgamma4 cells suppressed myocarditis. Adoptively transfusing enriched Vgamma4(+) cells to the C57BL/6 and Bl.Tg. Ealpha gammadelta ko strains confirmed that the Vgamma4 subset promoted myocarditis. Th subset analysis suggests that Vgamma1(+) cells biased the CD4(+) T cells to a dominant Th2 cell response, whereas Vgamma4(+) cells biased CD4(+) T cells toward a dominant Th1 cell response.     

2010年浙江省部分地区急性出血性 结膜炎暴发疫情病原学研究

为查明引起2010年浙江省急性出血性结膜炎(AHC)暴发疫情的病因,并对病原进行分子溯源。本研究采用荧光RT-PCR方法直接从患者眼拭子样本中检测肠道病毒(EV)和柯萨奇病毒A24变异株(CA24v)核酸;用Hep-2细胞分离病毒,对阳性分离物提取病毒核酸后进行VP1全基因和3C蛋白酶区(3C)扩增和测序,同源性与进化分析。结果13份眼拭子样本中EV和CA24v核酸均阳性8份,分离到CA24v6株。选取4株病毒测序,获得VP1全长均为915个核苷酸(nt),3C区全长495nt,VP1和3C区均没有nt插入和缺失。2010年浙江4株CA24v分离株之间在3C区和VP1区核苷酸和氨基酸(aa)高度同源,2010年浙江CA24v分离株与原型株EH24/70在3C区的nt和aa同源性分别为85.2%～85.8%和96.2%～96.7%,与2002～2008年浙江、云南和广东CA24v株的同源性分别为93.4%～96.2%和96.7%～99.3%;浙江2010年CA24v株在3C区进化树的GⅣ基因亚型C4分枝上(GⅣ-C4),在VP1基因进化树的人类肠道病毒C组(EV-C)CA24v分枝上。研究表明引起2010年浙江省急性出血性结膜炎暴发流行的病原为CA24v,GⅣ基因亚型,与引起2002～2008年浙江AHC流行的CA24v株(GⅣ)具有密切的亲缘关系,推测CA24v病毒自2002年以来一直在本地低强度循环,2010年又导致了浙江AHC的暴发。     

Cardiac myosin-induced myocarditis. Heart autoantibodies are not involved in the induction of the disease

We recently demonstrated that cardiac myosin is capable of inducing autoimmune myocarditis in genetically predisposed mice. This disease parallels coxsackievirus B3-induced autoimmune myocarditis in many respects and is associated with high-titer autoantibodies specific for cardiac myosin. The following lines of evidence suggest that these autoantibodies are not involved in the induction of autoimmune myocarditis: 1) immunoperoxidase staining of heart sections from cardiac myosin-immunized A/J and A.SW mice revealed IgG depositions only along damaged muscle fibres in infiltrated areas, but not in intact tissue; 2) myosin autoantibodies did not bind to the surface of viable cardiac myocytes isolated from mice, but only reacted with myocytes permeabilized with detergent; 3) mice treated with a single high dose of cyclophosphamide, which reduces the humoral immune response, still developed severe myocarditis, despite the fact that their autoantibody titers were reduced to the level of adjuvant-injected controls; and 4) passive transfer of high-titer myosin autoantibodies failed to induce myocarditis, although the titers in the recipients were comparable to those found in mice with cardiac myosin-induced disease. Together, the results suggest that high-titer myosin autoantibodies are secondary rather than primary to the disease.     

Dysferlin deficiency confers increased susceptibility to coxsackievirus‐induced cardiomyopathy

Coxsackievirus infection can lead to viral myocarditis and its sequela, dilated cardiomyopathy, which represent major causes of cardiovascular mortality worldwide in children. Yet, the host genetic susceptible factors and the underlying mechanisms by which viral infection damages cardiac function remain to be fully resolved. Dysferlin is a transmembrane protein highly expressed in skeletal and cardiac muscles. In humans, mutations in the dysferlin gene can cause limb‐girdle muscular dystrophy type 2B and Miyoshi myopathy. Dysferlin deficiency has also been linked to cardiomyopathy. Defective muscle membrane repair has been suggested to be an important mechanism responsible for muscle degeneration in dysferlin‐deficient patients and animals. Using both naturally occurring and genetically engineered dysferlin‐deficient mice, we demonstrated that loss of dysferlin confers increased susceptibility to coxsackievirus infection and myocardial damage. More interestingly, we found that dysferlin is cleaved following coxsackieviral infection through the proteolytic activity of virally encoded proteinases, suggesting an important mechanism underlying virus‐induced cardiac dysfunction. Our results in this study not only identify dysferlin deficiency as a novel host risk factor for viral myocarditis but also reveal a key mechanism by which coxsackievirus infection impairs cardiac function, leading to the development of dilated cardiomyopathy.     

Coxsackievirus group B type 3 infection upregulates expression of monocyte chemoattractant protein 1 in cardiac myocytes, which leads to enhanced migration of mononuclear cells in viral myocarditis

Coxsackievirus group B type 3 (CVB3) is an important cause of viral myocarditis. The infiltration of mononuclear cells into the myocardial tissue is one of the key events in viral myocarditis. Immediately after CVB3 infects the heart, the expression of chemokine(s) by infected myocardial cells may be the first trigger for inflammatory infiltration and immune response. However, it is unknown whether CVB3 can induce the chemokine expression in cardiac myocytes. Monocyte chemoattractant protein 1 (MCP-1) is a potent chemokine that stimulates the migration of mononuclear cells. The objective of the present study was to investigate the effect of CVB3 infection on MCP-1 expression in murine cardiac myocytes and the role of MCP-1 in migration of mononuclear cells in viral myocarditis. Our results showed that the expression of MCP-1 was significantly increased in cardiac myocytes after wild-type CVB3 infection in a time- and dose-dependent manner, which resulted in enhanced migration of mononuclear cells in mice with viral myocarditis. The migration of mononuclear cells was partially abolished by antibodies specific for MCP-1 in vivo and in vitro. Administration of anti-MCP-1 antibody prevented infiltration of mononuclear cells bearing the MCP-1 receptor CCR2 in mice with viral myocarditis. Infection by UV-irradiated CVB3 induced rapid and transient expression of MCP-1 in cardiac myocytes. In conclusion, our results indicate that CVB3 infection stimulates the expression of MCP-1 in myocardial cells, which subsequently leads to migration of mononuclear cells in viral myocarditis.     

川金丝猴体毛微量元素的分析

应用等离子发射光谱法分析了秦岭产川金丝猴体毛中Ｎａ、Ｋ、Ｃａ、Ｍｇ、Ｚｎ、Ｃｄ、Ｃｏ、Ｃｕ、Ｎｉ、Ｓｒ、Ｌｉ、Ｆｅ、Ａｌ、Ｍｎ、Ｂ、Ｐ１６种微量元素的含量,发现除Ｚｎ与Ｍｎ有显著的性别差异外,余者无显著的性别差异,一般雄性稍高于雌性。与四川产川金丝猴体毛中的Ｚｎ、Ｃａ、Ｃｕ、Ｆｅ含量比较,两地区样本均有极显著的差异。