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5-氟-2'-脱氧尿苷对佛罗里达州西南部水域中细菌浮游生物[h]胸苷掺入的影响。

Effect of 5-fluoro-2'-deoxyuridine on [h]thymidine incorporation by bacterioplankton in the waters of southwest Florida.

机构信息

Department of Marine Science, University of South Florida, 140 7th Avenue South, St. Petersburg, Florida 33701.

出版信息

Appl Environ Microbiol. 1988 Feb;54(2):331-6. doi: 10.1128/aem.54.2.331-336.1988.

Abstract

The effect of 5-fluoro-2'-deoxyuridine (FdUrd) on [methyl-H] thymidine incorporation by bacterioplankton populations in subtropical freshwater, estuarine, and oceanic environments was examined. In estuarine waters, intracellular isotope dilution was inhibited by FdUrd, which enabled us to estimate both intracellular and extracellular isotope dilution. In 2 of 10 cases, extracellular isotope dilution was significant. At low concentrations of [methyl-H]thymidine or [6-H]thymidine, FdUrd completely inhibited incorporation of radioactivity into protein and RNA. At high concentrations of [H]thymidine, however, FdUrd had little effect on labeling patterns. The dihydrofolate reductase inhibitors amethopterin and trimethoprim had no effect on macromolecular labeling patterns. These results suggest that thymidylate synthase is not involved in nonspecific labeling and that FdUrd inhibits nonspecific labeling by blocking some other enzyme involved in thymidine catabolism. In oligotrophic oceanic and freshwater samples, FdUrd did not inhibit intracellular isotope dilution or [H]thymidine labeling of protein and RNA, but caused some inhibition of [H]thymidine incorporation into DNA. The ability of FdUrd to inhibit nonspecific macromolecular labeling during [H]thymidine incorporation was significantly correlated (r = 0.84) with total thymidine incorporation (in picomoles per liter per hour). The results are discussed in terms of applications of FdUrd to routine bacterial production measurements and the general assumptions of [H]thymidine incorporation.

摘要

研究了 5-氟-2'-脱氧尿苷(FdUrd)对亚热带淡水、河口和海洋环境中细菌浮游生物种群中[甲基-H]胸苷掺入的影响。在河口水中,FdUrd 抑制了细胞内同位素稀释,这使我们能够估计细胞内和细胞外的同位素稀释。在 10 个案例中的 2 个案例中,细胞外同位素稀释是显著的。在[甲基-H]胸苷或[6-H]胸苷的低浓度下,FdUrd 完全抑制放射性活性掺入蛋白质和 RNA 中。然而,在[H]胸苷的高浓度下,FdUrd 对标记模式几乎没有影响。二氢叶酸还原酶抑制剂氨蝶呤和三甲氧苄氨嘧啶对大分子标记模式没有影响。这些结果表明胸苷酸合成酶不参与非特异性标记,并且 FdUrd 通过阻断参与胸苷分解代谢的其他一些酶来抑制非特异性标记。在贫营养海洋和淡水样本中,FdUrd 不抑制细胞内同位素稀释或[H]胸苷标记蛋白质和 RNA,但会导致[H]胸苷掺入 DNA 的一些抑制。FdUrd 在[H]胸苷掺入期间抑制非特异性大分子标记的能力与总胸苷掺入(每升每小时皮摩尔)显著相关(r = 0.84)。结果根据 FdUrd 在常规细菌产量测量中的应用和[H]胸苷掺入的一般假设进行了讨论。

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