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添加到酸化琼脂培养基中的血液和木炭可促进日内瓦分枝杆菌的生长。

Blood and charcoal added to acidified agar media promote the growth of Mycobacterium genavense.

作者信息

Realini L, De Ridder K, Hirschel B, Portaels F

机构信息

Department of Microbiology, Mycobacteriology Unit, Institute of Tropical Medicine, Antwerp, Belgium.

出版信息

Diagn Microbiol Infect Dis. 1999 May;34(1):45-50. doi: 10.1016/s0732-8893(99)00014-0.

Abstract

Ten different agar media were tested for the in vitro growth of Mycobacterium genavense in primary cultures and in subcultures from BACTEC vials. These agar media were based on Middlebrook 7H9, 7H10 and 7H11, and supplemented with additives: mycobactin J, yeast extract, charcoal, or defibrinated sheep blood. Some media were acidified with phosphoric acid to a final pH of 6.2 +/- 0.2. Fourteen M. genavense strains from nude mouse organs as well as one decontaminated clinical specimen (from a bird) were tested. The optimal medium for primary cultures of M. genavense was Middlebrook 7H11 acidified to pH 6.2 +/- 0.2 and supplemented with charcoal and sheep blood: on this medium, all strains produced colonies within 6-12 weeks of incubation in numbers approaching the number of bacilli inoculated. It was also the only medium to support the growth of the decontaminated clinical specimen. Added blood and charcoal appeared not as essential for subcultures as for primary cultures. Three media supported the growth of all strains within 1 month incubation: they were acidified, and were supplemented with yeast extract or pancreatic digest of casein, and with either blood or charcoal.

摘要

对10种不同的琼脂培养基进行了测试,以观察日内瓦分枝杆菌在原代培养物以及来自BACTEC瓶的传代培养物中的体外生长情况。这些琼脂培养基以Middlebrook 7H9、7H10和7H11为基础,并添加了添加剂:分枝杆菌素J、酵母提取物、活性炭或去纤维羊血。一些培养基用磷酸酸化至最终pH值为6.2±0.2。对来自裸鼠器官的14株日内瓦分枝杆菌菌株以及1份经净化的临床标本(来自一只鸟)进行了测试。日内瓦分枝杆菌原代培养的最佳培养基是酸化至pH值6.2±0.2并添加了活性炭和羊血的Middlebrook 7H11:在这种培养基上,所有菌株在培养6 - 12周内都形成了菌落,数量接近接种的杆菌数量。它也是唯一能支持经净化的临床标本生长的培养基。对于传代培养而言,添加的血液和活性炭似乎不像原代培养那样必不可少。有三种培养基在培养1个月内支持了所有菌株的生长:它们经过酸化处理,并添加了酵母提取物或酪蛋白胰酶消化物,以及血液或活性炭。

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