• 主题
高级搜索  >
历史搜索 清空历史
首页> 外文期刊>Biologicals: Journal of the International Association of Biological Standardization >Nutritional effects of culture media on mycoplasma cell size and removal by filtration.
【24h】

Nutritional effects of culture media on mycoplasma cell size and removal by filtration.

机译:培养基对支原体细胞大小的营养影响,并通过过滤去除。

获取原文
获取原文并翻译 | 示例
页面导航
  • 摘要
  • 著录项
  • 相似文献
  • 相关主题

摘要

Careful media filtration prior to use is an important part of a mycoplasma contamination prevention program. This study was conducted to increase our knowledge of factors that influence efficient filtration of mycoplasma. The cell size of Acholeplasma laidlawii was measured after culture in various nutritional conditions using scanning electron microscopy. The maximum cell size changed, but the minimum cell size remained virtually unchanged and all tested nutritional conditions resulted in a population of cells smaller than 0.2 microm. Culture in Tryptic Soy Broth (TSB) resulted in an apparent increase in the percentage of very small cells which was not reflected in increased penetration of non-retentive 0.2 microm rated filters. A. laidlawii cultured in selected media formulations was used to challenge 0.2 microm rated filters using mycoplasma broth base as the carrier fluid. We used 0.2 microm rated filters as an analytical tool because A. laidlawii is known to penetrate 0.2 microm filters and the degrees of penetration can be compared. Culture of A. laidlawii in TSB resulted in cells that did not penetrate 0.2 microm rated filters to the same degree as cells cultured in other media such as mycoplasma broth or in TSB supplemented with 10% horse serum.
机译:使用前仔细过滤培养基是预防支原体污染计划的重要组成部分。进行这项研究是为了增加我们对影响支原体有效过滤的因素的认识。在各种营养条件下培养后,使用扫描电子显微镜测量了无毛破壁虫的细胞大小。最大细胞大小发生了变化,但最小细胞大小却基本保持不变,所有测试的营养条件均导致细胞群体小于0.2微米。胰蛋白酶大豆肉汤(TSB)中的培养导致非常小的细胞百分比明显增加,这未反映在非保持性0.2微米额定过滤器的渗透增加中。使用支原体肉汤基质作为载液,使用在选定培养基配方中培养的A. lawlawii攻击0.2微米级滤膜。我们使用0.2微米等级的过滤器作为分析工具,因为已知A. Ladlawii可以穿透0.2微米的过滤器,并且可以比较穿透程度。在TSB中培养A. lawlawii导致细胞无法穿透0.2微米等级的滤膜,其程度与在其他培养基(如支原体肉汤)或添加了10%马血清的TSB中培养的细胞相同。

著录项

相似文献

  • 外文文献
  • 中文文献
  • 专利
获取原文

客服邮箱:kefu@zhangqiaokeyan.com

京公网安备:11010802029741号 ICP备案号:京ICP备15016152号-6 六维联合信息科技 (北京) 有限公司©版权所有

  • 客服微信

  • 服务号