H5N1接种恒河猴和食蟹猴后外周血细胞变化的分析

目的测定H5N1型禽流感病毒感染恒河猴、食蟹猴后,其外周血细胞的变化,为H5N1模型猴提供基础数据及研究参考。方法健康合格食蟹猴、恒河猴各4只,经滴鼻方式接种H5N1病毒107TCID50,确认发病后,在不同时间点进行血细胞及T淋巴细亚群的分析。结果与接种H5N1病毒前比较,接种后白细胞总数（WBC）在第6天时有所降低,至第9天时回升;红细胞总数（RBC）在第3天有所降低,之后回升;淋巴细胞比例及数量分别在第6天、第9天升高并达到最高值。至第9天时,CD4^＋T细胞数明显高于接种前,CD8^＋T细胞数上升显著,导致CD4^＋/CD8^＋T细胞比例下降,甚至在2只食蟹猴出现了比例倒置。结论实验用猴感染H5N1后,可导致WBC,CD4^＋,CD8^＋T等血液细胞的变化,应作为H5N1模型动物的检测指标。     

BALB/c小鼠和雪貂感染H7N9禽流感病毒后的肺组织动态病理学变化

目的了解用H7N9禽流感病毒分别感染BALB/c小鼠和雪貂后,其肺部动态病理改变,为临床诊断、治疗、预防及机制研究提供帮助。方法 BALB/c小鼠经鼻腔接种106EID50(50μL)H7N9禽流感病毒后第1、2、3、5、7、14、28天分别安乐死2~3只小鼠;雪貂经鼻腔吸入接种106EID50(500μL)H7N9禽流感病毒后第3、7、14、28天分别安乐死1只雪貂,分别观察动物的临床特征改变,肺组织的大体组织形态学变化,HE染色观察动态病理改变,免疫组化染色观察病毒分布及肺组织各种炎细胞的浸润情况。结果感染病毒后的小鼠出现竖毛、嗜睡、死亡等表现,雪貂表现为打喷嚏、鼻腔分泌物、稀便、嗜睡等;大体观察小鼠与雪貂肺组织均可见到暗红色病灶;光镜观察小鼠与雪貂的肺组织均呈现坏死性支气管炎和渗出性间质性肺炎、肺泡炎。感染第2天开始出现炎性病变,7~9 d炎症病变最严重,14 d后逐渐修复吸收,28 d基本完全吸收;T、B淋巴细胞,巨噬细胞不同程度的表达增多,以T细胞增多为主,尤其是CD8+T细胞两种动物均大量表达。结论 H7N9禽流感病毒感染可引起BALB/c小鼠和雪貂肺组织急性支气管炎和肺炎,感染后7~9 d肺部炎症的组织病理学变化最严重,CD8+T细胞明显增多,14d后病灶逐渐吸收。该研究可为临床诊断、治疗、预防该病及进行疾病机制研究提供帮助。     

虎源H5N1亚型禽流感病毒感染小鼠模型的建立

为研究H5N1亚型禽流感病毒的病原特性、致病机理及对其疫苗与救治药物效果评价提供平台,利用本室分离鉴定的虎源A/Tiger/Harbin/01/2002株(简称HAB/01)H5N1亚型禽流感病毒进行连续10倍稀释后,对4～6周龄雄性BALB/c小鼠经乙醚麻醉后进行滴鼻攻毒,每个稀释度接种10只实验小鼠,测定其MLD50,检测小鼠感染、致病的多项指标,观察期为14d。结果感染小鼠呈现出规律的以肺炎为主的临床症状、病理变化及病死率;测得该病毒对小鼠的MLD50为10-7.1/0.05mL。成功建立了虎源H5N1亚型禽流感病毒感染BALB/c小鼠的实验模型。     

虎源H5N1亚型禽流感病毒感染小鼠模型的建立

为研究H5N1亚型禽流感病毒的病原特性、致病机理及对其疫苗与救治药物效果评价提供平台,利用本室分离鉴定的虎源A/Tiger/Harbin/01/2002株(简称HAB/01)H5N1亚型禽流感病毒进行连续10倍稀释后,对4～6周龄 雄性BALB/c小鼠经乙醚麻醉后进行滴鼻攻毒,每个稀释度接种10只实验小鼠,测定其MLD50,检测小鼠感染、致病的多项指标,观察期为14d.结果感染小鼠呈现出规律的以肺炎为主的临床症状、病理变化及病死率;测得该病毒对小鼠的MLD50为10-7.1/0.05mL.成功建立了虎源H5N1亚型禽流感病毒感染BALB/c小鼠的实验模型.     

禽流感H5N1亚型病毒感染ICR小鼠模型建立

[目的]建立H5N1禽流感病毒感染ICR小鼠的模型;[方法]ICR小鼠鼻腔接种H5N1禽流感病毒,观察其接毒后的症状、体征、体重和体温的变化;取材分离病毒和制作病理,用ELISA的方法检测血清抗体;[结果]接受感染ICR小鼠表现出一系列的症状和体征,其活动明显减少,反应性差,体温和体重快速下降;在小鼠的肺、脑、气管和心、肝、脾、肾都可分离到病毒。ICR小鼠的死亡率为60%。ICR小鼠的肺部病变最严重,表现为间质性肺炎,肺间质充血、水肿和淋巴细胞浸润;血管周围淋巴细胞浸润,毛细血管扩张;上皮细胞变性、坏死、脱落,并有充血和单核细胞浸润;肺…     

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。     

H7N9禽流感病毒小鼠感染动物模型的建立

目的建立H7N9禽流感病毒小鼠感染模型。方法 1×108,1×107或1×106TCID50H7N9禽流感病毒原液(A/Anhui/1/2013)滴鼻感染BALB/c小鼠。主要观测指标:临床症状、死亡率、病理变化、病毒载量和血清抗体检测。结果被感染的小鼠表现为竖毛、弓背、体重下降;病理表现为间质性肺炎,感染后第2天开始在呼吸道脱落细胞中检测到病毒;免疫组化或病毒分离方法在肺、肾、脑、肠、脾等组织检测到病毒;感染后14 d在小鼠血清中血凝抑制试验特异性抗体效价达到160;淋巴细胞减少,中性粒细胞增多。结论 H7N9感染BALB/c小鼠模型与人类禽流感感染疾病的基本特征相似,为研究该病的发病机制及药物疫苗的研发提供了工作基础。     

禽流感H5N1病毒不同途径感染BALB/c小鼠的临床和病理比较

我们将禽流感H5N1病毒通过鼻腔、尾静脉和脑内接种方式接种BALB/c小鼠,观察小鼠在感染过程中临床症状和各个组织器官的病理变化。感染1天后,小鼠打堆、猥琐、毛色混乱、眼角有分泌物;感染第2天的小鼠均出现死亡;感染4天后,小鼠从临床症状上表现恢复。收集各种方式感染的小鼠的主要脏器进行组织病理学检查,结果显示,小鼠不同接种途径感染H5N1流感病毒后,所产生的病理变化相似;从各个脏器的病变程度来看,病毒最先到达的器官损伤最严重。感染第2天各组织器官的病变最严重,随着感染时间增长,肺脏和肾脏等器官有不同程度的恢复,心脏和肝脏等器官的病变在感染过程中未见明显恢复。     

近年来华东地区家鸭中禽流感病毒的亚型分布

[目的]为了研究近年来华东地区家鸭中禽流感病毒的亚型分布情况.[方法]对2002-2006年分离自华东地区家鸭的180株禽流感病毒的HA亚型和其中88株禽流感病毒的NA亚型分别进行了测定.[结果]近年来华东地区家鸭中至少存在9种HA亚型和6种NA亚型组成的H1N1,H3N1,H3N2,H3N8,H4N6,H5N1,H5N2,H6N2,H6N8,H8N4,H9N2,H10N3,H11N2共13种亚型的禽流感病毒.[结论]华东地区家鸭中有多种亚型的禽流感病毒分布,应加强家鸭禽流感的监测和防制工作.     

禽流感H5N1亚型病毒感染ICR小鼠的动物模型

目的 建立H5N1禽流感病毒感染ICR小鼠的疾病动物模型.方法 将100 μL H5N1 禽流感病毒原液(EID50为105.37/0.2 mL) 鼻腔接种ICR小鼠,设生理盐水组、正常尿囊液组对照,接毒后14 d内每隔12 h观察一次,主要观测指标有临床体征、体重和体温变化、死亡率、病理变化、病毒分离和血清抗体检测 (ELISA方法).结果 被感染的ICR小鼠的病程可以划分为潜伏期 (第0～1天)、急性感染期 (第2～7天)、恢复期 (第8～14天),急性感染期表现出活动明显减少,弓背,反应性差,扎堆;接毒后第1天开始体温和体重下降,第6天体温和体重停止下降;接毒组ICR小鼠累计的死亡率为60%;急性感染期ICR小鼠的肺部病变最严重,表现为间质性肺炎,肺间质充血、水肿和淋巴细胞浸润,毛细血管扩张,上皮细胞变性、坏死、脱落,并有充血和单核细胞浸润;接毒后第1天至第8天可在小鼠的肺、脑、气管和心、肝、脾、肾分离到病毒;接毒后第6天从ICR小鼠血清中检测到抗体.结论 本实验室建立的H5N1禽流感病毒感染ICR小鼠的模型在临床表现、体重变化、死亡率、病理变化、病毒复制指标能达到禽流感病毒疾病模型的造模要求,符合人类禽流感感染疾病的基本特征.     

Root Colonization by Inoculated Plant Growth-Promoting Rhizobacteria

Certain rhizobacteria referred to as 'plant growth-promoting rhizobacteria' (PGPR) can contribute to the biological control of plant pathogens and improve plant growth. They enhance root development either directly by producing phytohormones, or indirectly by inhibiting pathogens through the synthesis of different compounds. PGPR are likely to be of great interest in sustainable crop protection and have drawn much attention in recent years. However, the use of these bacteria to protect crops sometimes fails because rhizobacteria are unable to recolonize the rhizosphere of inoculated plants. The colonization of roots by inoculated bacteria is an important step in the interaction between beneficial bacteria and the host plant. However, it is a complex phenomenon influenced by many biotic and abiotic parameters, some of which are now apparent. This paper summarises knowledge on rhizosphere colonization by PGPR.     

Inoculated mouse model of Pneumocystis carinii pneumonia.

A transtracheally inoculated mouse model of Pneumocystis carinii has been developed using BALB/c mice, a widely available strain free of latent P. carinii infection. The mean infectivity score of untreated inoculated mice was 4.1 compared to the mean infectivity score of 0.1 for trimethoprim/sulfamethoxazole (50/250 mg/kg) treated inoculated mice, approximately a four-log difference. An inoculated mouse model of P. carinii infection provides both a source of organisms from a different host and an animal model for study of drugs for therapy and prophylaxis which is less costly than rats and which requires less drug than required for rats.     

Metabolism of Barley Leaves Inoculated with Erysiphe graminis Merat

Inoculating Proctor barley leaves with Erysiphe graminis decreasedrates of photosynthesis, after an initial lag period, and increasedrespiration. Increasing the area inoculated progressively decreased ratesof photosynthesis, but the effects cannot be attributed to asimple loss of leaf area. When less than 30 per cent of a leafwas inoculated, decreases were equivalent to area losses greaterthan those inoculated; when more than 30 per cent was inoculatedthe photo-synthetic losses were equivalent to area losses lessthan those inoculated. Although the relative effects of E. graminis on photosynthesisand respiration were of the same order, the absolute effectson photosynthesis were greater than those on respiration. Inoculating30 per cent of a leaf decreased photosynthesis by 5–6mg CO₂/dm²/hr from 12.9 in the uninoculated controls to 7.3.Respiration increased by 0.6 mg CO₂/dm/hr, from 1.7 to 2.3-     

Leakage from Seedling Roots, Inoculated with Phytophthora cinnamomi

A sequential study of electrolyte leakage from roots inoculated with Phytophthora cinnamomi demonstrated changes in leakage in response to infection. These changes may be characterised in terms of susceptibility and resistance. Field resistant species showed two types of response (i) rapid leakage 2—4 h after inoculation, such as in Eucalyptus calophylla, E. maculata and Gahnia radula, (ii) no significant increase in leakage with infection, for example in cereals and in juncus bufonius. Susceptible species, such as Xanthorrhoea australis, E. sieberi and E. marginata showed slow but continually increasing leakage after inoculation, and usually lost significantly more electrolyte than field resistant species. Both electrolyte leakage and susceptibility of two Eucalyptus species varied with root temperature. Roots of both the susceptible and field resistant Eucalyptus species grown at 14°C showed similar leakage patterns to those grown at 24°C although no lesions formed at 14°C. Both amount of leakage and lesion length increased at 28°C. E. marginata (susceptible) lost significantly greater quantities of electrolyte than E. calophylla at each temperature tested. Leakage from artificially wounded roots did not vary with either temperature or with host susceptibility. No significant changes in conductivity were recorded with saprophytic colonization of roots, or with incubation in either low molecular weight culture filtrate or β-glucan solutions. Vacuum infiltration with the culture filtrate or the β-glucan slightly increased initial electrolyte loss in comparison with that of the controls. The increased leakage from infected roots may be toxin mediated or due to enzymie degradation of host plasma membranes, and occurred within the region of the limited lesion in the case of field resistant species, compared with the larger zone of extending necrosis characteristic of susceptible species.     

Observations on Eimeria tenella in Feces of Inoculated Chickens

SYNOPSIS. In studies on coccidial excystation, Eimeria tenella sporulated oocysts were fed to 5 individually caged chickens, and during the next 4.5 hours, all droppings were collected immediately after excretion, mixed with 0.85% NaCl solution, then promptly examined for the parasites. Some samples were placed in cold storage at 4 C and examined at intervals thereafter. Three of the birds were necropsied after 5 hours and the intestinal contents examined. Apparently unbroken oocysts containing active sporozoites were in chicken droppings beginning 1–2.25 hours postinoculation; some activated forms were inside and others outside the sporocysts. Free sporozoites, sometimes numerous, first appeared in the feces 1.1–2 hours postinoculation. At necropsy, the state and condition of the parasites in the lumen of bird intestines were similar to those in its last fecal dropping. After being in cold storage for 48 hours, free sporozoites inside and outside the oocysts became active and moved about when placed on the warming stage of the microscope.     

Comparative Volatile Profiles in Soy Sauce According to Inoculated Microorganisms

We compared the volatile profiles in soy sauce according to inoculation with Tetragenococcus halophilus and/or Zygosaccharomyces rouxii. Totals of 107 and 81 volatiles were respectively identified by using solid-phase microextraction and solvent extraction. The various volatile compounds identified included acids, aldehydes, esters, ketones, furans and furan derivatives, and phenols. The major volatiles in the samples treated with T. halophilus were acetic acid, formic acid, benzaldehyde, methyl acetate, ethyl 2-hydroxypropanoate, 2-hydroxy-3-methyl-2-cyclopenten-1-one, and 4-hydroxy-3-methoxybenzaldehyde, while those in the samples inoculated with Z. rouxii were mainly ethanol, acetaldehyde, ethyl propanoate, 2/3-methylbutanol, 1-butanol, 2-phenylethanol, ethyl 2-methylpropanoate, and 4-hydroxy-2-ethyl-5-methyl-3(2H)-furanone. The results indicate that T. halophilus produced significant acid compounds and could affect the Z. rouxii activity, supporting the notion that yeasts and lactic acid bacteria respectively have different metabolic pathways of alcoholic fermentation and lactic acid fermentation, and produce different dominant volatile compounds in soy sauce.     

Changes in Respiration of Seedling Roots Inoculated with Phytophthora cinnamomi

An increase in rate of respiration was recorded for intact roots of seven native Australian species 16 h after inoculation with Phytophthora cinnamomi. By 24 h the magnitude of the increase ranged from 2—159% above that of the uninoculated controls and was evidently not related to host susceptibility. A time sequence study of lesion extension and the associated increased respiration rates for both susceptible and tolerant eucalypts demonstrated a difference in response. The rate of respiration in the tolerant species increased 2 % and only at the site of inoculation, whereas in the susceptible species the respiration rate increased in a wave which began at the inoculation site and continued along the root with the advancing fungal invasion. Respiration rate only increased in regions of the root actually inhabited by the pathogen. The fungal contribution to the total respiration of infected roots was less than 1 % and was determined by measuring respiration of inoculated killed roots. Respiration rates were measured in the presence of potassium cyanide (KCN) and salicylhydroxamic acid (SHAM). Both KCN-sensitive and SHAM-sensitive respiration occurred in normal uninfected E. marginate seedlings. A large proportion of the increase in total respiration rate of infected seedlings compared with uninoculated controls was due to the alternate, SHAM-sensitive pathway. The physiological implications of these results are discussed.     

Removal of Phthalate Esters in Soil Column Inoculated with Microorganisms

The removal of phthalate esters, such as di-2-ethyl hexyl phthalate (DEHP) was efficiently effected by inoculating and retaining viable cells of Nocardia erythropolis, a bacterium known capable of rapidly degrading phthalate esters, in soil column. When an influent containing 3000 ppm of DEHP was passed through a column inoculated with Nocardia erythropolis, the eluent from the column was gas-chromatographically free of DEHP after 1 day. Residual DEHP on the support after 32 days in the column inoculated with Nocardia erythropolis was only 0.14% against the total amount of DEHP fed, whereas it was 5.2% in the uninoculated column. Microorganisms capable of utilizing DEHP were isolated from the inoculated and un- inoculated columns after 32 days operation and identified. The DEHP utilizing microorganisms in the inoculated column were found to belong to Nocardia erythropolis, Nocardia restricta and Pseudomonas putida (Biotype B), and those in the uninoculated column to Nocardia erythropolis, Pseudomonas putida (Biotype A and B) and Pseudomonas acidovorans. In particular, strain 1-1 of Nocardia erythropolis isolated from the inoculated column was morphologically and biochemically identical with the inoculated Nocardia erythropolis S-l. Ratio of all Nocardia erythropolis to total cells recovered increased from 10.8% immediately after inoculation to 27.2% after 32 days in inoculated column.