肺炎支原体与仓鼠气管器官培养物、气管外植单层细胞、人红细胞及WiDr人组织培养细胞的黏附。
Attachment of Mycoplasma pneumoniae to hamster tracheal organ cultures, tracheal outgrowth monolayers, human erythrocytes, and WiDr human tissue culture cells.
作者信息
Chandler D K, Collier A M, Barile M F
出版信息
Infect Immun. 1982 Mar;35(3):937-42. doi: 10.1128/iai.35.3.937-942.1982.
Abstract
Virulent strains of Mycoplasma pneumoniae, PI-1428 and M129, were radiolabeled wtih [3H]palmitic acid or [3H]thymidine and examined for attachment to hamster tracheal organ cultures, tracheal outgrowth monolayers, human O-positive erythrocytes, and human WiDr carcinoma cell cultures. Although attachment to each cell substrate was readily detected, the WiDr cell culture monolayers provided the most satisfactory substrate for quantitating mycoplasma attachment. Serious technical limitations were encountered with each of the other substrates that we examined; these limitations interfered with reproducibility or sensitivity and rendered tracheal organ cultures and erythrocyte suspensions unsuitable for routine attachment and attachment inhibition assays. Moreover, the WiDr cell monolayer was the most sensitive substrate for determining attachment inhibition activity in protein-containing extracts prepared from M. pneumoniae. The significance of these findings is discussed.
摘要
肺炎支原体的强毒株PI - 1428和M129用[3H]棕榈酸或[3H]胸苷进行放射性标记,并检测其对仓鼠气管器官培养物、气管外植体单层、人O型阳性红细胞和人WiDr癌细胞培养物的附着情况。虽然很容易检测到支原体对每种细胞底物的附着,但WiDr细胞培养单层为定量支原体附着提供了最理想的底物。我们检测的其他每种底物都遇到了严重的技术限制;这些限制干扰了重现性或敏感性,使得气管器官培养物和红细胞悬液不适用于常规的附着和附着抑制试验。此外,WiDr细胞单层是测定肺炎支原体制备的含蛋白质提取物中附着抑制活性最敏感的底物。讨论了这些发现的意义。
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