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首页> 外文期刊>Revista de Biología Tropical >Aislamiento de una cepa de campo de Babesia bigemina (Piroplasma: Babesiidae) y establecimiento del cultivo in vitro para la producción de antígenos
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Aislamiento de una cepa de campo de Babesia bigemina (Piroplasma: Babesiidae) y establecimiento del cultivo in vitro para la producción de antígenos

机译:分离出大巴贝斯虫(Babesia bigemina)田间菌株(Piroplasma:Babesiidae)并建立用于产生抗原的体外培养

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Isolation of a field strain of Babesia bigemina (Piroplasma: Babesiidae) and establishment of in vitro culture for antigen production. Bovine babesiosis, caused by Babesia bigemina, is a barrier for livestock development; it results in high economic loss to Mexican livestock. Control requires adequate antigens for diagnosis and vaccination programs. However, because of antigenic variation among Babesia strains, it is necessary to use antigens prepared from local strains. The purpose of the present study was to isolate a local field strain and to establish the in vitro culture of B. bigemina by the evaluation of the constituent?s concentration of culture media. Thirty engorged female Boophilus microplus were collected from cattle suffering clinical babesiosis (B. bigemina) in Yucatan state, Mexico. These ticks were sent to the laboratory for detection of Babesia sp. vermicules. Eggs were kept at 83-85 % humidity and 27 oC until hatching. Larvae were transferred to an esplenectomized calf (B-1). The resulting nymphs were transferred to an esplenectomized calf (B-2). Twelve days later, B. bigemina (local strain) was detected in calf B-2 and its infected blood was frozen in liquid nitrogen to initiate the in vitro culture. The Microaerophilus Stationary Phase (MASP) in vitro culture method was used to reactivate the parasite. Three different concentrations of culture media (70, 60 and 50 %), serum (30, 40 and 50 %) and uninfected red blood cells (5, 10 and 15 %) were used in order to know the convenient concentrations to obtain the highest percentage of infected red blood cells (PEI). The cultured strain was used to prepare antigens for the Immunofluorescence Antibody Test (IFAT) and several concentrations of serum and conjugate were tested. Strain isolation was successful; 30 days were needed to obtain a PEI of 1.5 %. The isolated strain was frozen in liquid nitrogen and the parasites were reactivated with the in vitro culture MASP method. The concentration of culture media that produced the highest PEI (14 %) (p
机译:分离出大巴贝斯虫(Babesia bigemina)(Piroplasma:Babesiidae)的田间菌株,并建立用于抗原产生的体外培养。大巴贝虫病引起的牛杆状杆菌病是畜牧业发展的障碍。这给墨西哥的牲畜造成了巨大的经济损失。控制需要足够的抗原用于诊断和疫苗接种程序。然而,由于巴贝斯氏菌菌株之间的抗原变异,因此有必要使用由局部菌株制备的抗原。本研究的目的是通过评估培养基中的成分浓度来分离本地野外菌株并建立大双歧杆菌的体外培养。从墨西哥尤卡坦州患有临床巴贝氏菌病(B. bigemina)的牛中收集了三十只饱满的雌性Boophilus microplus。这些壁虱被送往实验室检测巴贝斯虫。 mic头。将卵保持在83-85%的湿度和27 oC直至孵化。将幼虫转移至脾切除的小牛(B-1)。将得到的若虫转移到脾切除的小牛(B-2)。 12天后,在小牛B-2中检测到了B. bigemina(本地菌株),并将其感染的血液冷冻在液氮中以启动体外培养。使用微嗜氧菌静止期(MASP)体外培养方法重新激活寄生虫。使用三种不同浓度的培养基(70%,60%和50%),血清(30%,40%和50%)和未感染的红细胞(5%,10%和15%),以了解获得最高浓度的方便浓度被感染的红细胞(PEI)的百分比。培养的菌株用于制备免疫荧光抗体测试(IFAT)的抗原,并测试了几种浓度的血清和结合物。应变隔离成功;需要30天才能获得1.5%的PEI。分离出的菌株在液氮中冷冻,并通过体外培养MASP方法重新激活寄生虫。产生最高PEI(14%)(p

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