畜牧兽医学报 ›› 2019, Vol. 50 ›› Issue (4): 851-860.doi: 10.11843/j.issn.0366-6964.2019.04.018

• 预防兽医 • 上一篇    下一篇

鉴别显色培养基在奶牛乳房炎病原菌快速鉴定中的应用

吕天星, 李松建, 郝永清*   

  1. 内蒙古农业大学兽医学院微生物学与免疫学实验室, 呼和浩特 010018
  • 收稿日期:2018-09-06 出版日期:2019-04-23 发布日期:2019-04-23
  • 通讯作者: 郝永清,主要从事微生物与免疫学研究,E-mail:haoyq1960@163.com
  • 作者简介:吕天星(1990-),男,内蒙古赤峰人,博士生,主要从事微生物与免疫学研究,E-mail:zeizhuai1@163.com
  • 基金资助:

    国家自然科学基金(31460664)

Application of a New On-farm Differential Chromogenic Medium for Fast Identification of Pathogens Associated with Mastitis in Milk of Dairy Cows

LÜ Tianxing, LI Songjian, HAO Yongqing*   

  1. Laboratory of Microbiology and Immunology, College of Veterinary Medicine, Inner Mongolia Agricultural University, Hohhot 010018, China
  • Received:2018-09-06 Online:2019-04-23 Published:2019-04-23

摘要:

为研发用于奶牛乳房炎常见病原菌分离鉴定的鉴别显色培养基,并检验其与普通分离鉴定培养基辅以生化鉴定和16S rRNA核酸序列测定两种传统方法鉴定结果的一致性,笔者以生物信息学方法筛出各种属细菌的特异性酶、可作为唯一碳源发酵产酸的碳源,然后合成酶显色底物,连同碳源、酸碱指示剂制备显色培养基,将各种属标准菌株、野生型菌株涂布培养,评估菌落形态、菌落颜色及培养基基质颜色变化。采集隐性乳房炎(CMT法检测)及临床型乳房炎病例的牛奶样品(絮状物、凝块、清亮状或血乳)共计482份,用鉴别显色培养基和两种传统方法进行病原菌的分离、鉴定。鉴别显色培养基上菌落纯化后提取DNA用于16S rRNA序列扩增,产物送去测序(n=194)。以两种传统方法为参考,判定鉴别显色培养基鉴定病原菌的可靠性,用SAS 9.4的FREQ程序计算鉴别显色培养基的简单科恩κ系数。鉴别显色培养基上常见乳房炎病原菌不同种属的菌落形态和培养基基质颜色明显不同,肉眼即可辨别。鉴别显色培养基与两种传统方法鉴定结果的一致性参数分别为κ=0.70、κ=0.96。鉴别显色培养基能够作为常见奶牛乳房炎病原菌的标准鉴定方法。

关键词: 奶牛, 乳房炎, 病原菌快速鉴定, 鉴别显色培养基

Abstract:

The present study aimed to develop a new differential chromogenic medium for fast identification of pathogens associated with mastitis in dairy cows, and check its identification consistency with two traditional approaches including normal isolation and identification media combined with biochemical identifications and 16S rRNA sequencing. Specific enzymes and the only carbon source that could be used to produce acid in bacteria of each genus were screened via bioinformatics tools. Synthesized chromogenic substrate of specific enzyme, carbon and acid-base indicator were mixed into basal enrichment medium to prepare differential chromogenic media. Standard strains and wild-type strains of related pathogens were inoculated on differential chromogenic media, and morphology of colonies and color changes of colony and medium that could be considered as identification standards were observed. Milk samples from mastitic quarters (samples diagnosed as subclinical mastitis by California Mastitis Test or samples of clinical mastitis with presence of flakes, clots, or serous milk; n=482) were cultured aerobically at 37℃ and identified using differential chromogenic media and traditional culture methods. Colonies from differential chromogenic media were purified and DNA was extracted for 16S rRNA sequencing (n=194). The reliability of identification by differential chromogenic media was diagnosed referring to results of two traditional approaches, based on which consistency inspection parameter, namely, simple Cohen's kappa coefficient was calculated via FREQ program in SAS Version 9.4. The colony and color of medium matrix from common bovine mastitis-associated pathogens of different genus grown on differential chromogenic media, regardless of standard strains or wild-type strains, were morphologically distinct and visible to the naked eyes. Consistency inspection parameter of differential chromogenic media referred to normal isolation and identification media combined with biochemical identifications and 16S rRNA sequencing was seperately κ=0.70 and κ=0.96. In conclusion, differential chromogenic media showed great potential in identifying common pathogens of bovine mastitis.

Key words: dairy cow, mastitis, fast identification of pathogens, differential chromogenic medium

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