发光酶基因标记荧光假单胞菌X16L2的发光研究
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*国家自然科学基金(批准号:39570028);国际科学基金(批准号:C/2362-1);湖北省自然科学基金,95J14


BIOLUMINESCENCE OF LUXAB-GENES-MARKED PSEUDOMONAS FLUORESCENS X16L2
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    摘要:

    通过发光光度仪和AMPN法定量测定荧光假单胞菌X16LZ(Pseudomonas fluorescens X16L2,简称X16L2)在液培和土壤中的发光情况及其数量,发现X16L2在液培和土壤中的发光动力学曲线相似,达到稳定发光强度的时间均在加入反应底物癸醛后约7分钟.X16L2在液培中的发光强度与生物量呈正相关.土壤中X16L2的发光量既与活菌数有关,也与土壤条件有关.土著微生物对X16L2的发光量、发光潜势和存活性有很大影响.本项研究表明,在一般情况下发光强度定量法既可对样品中标记微生物的生理活性进行原位快速测定,又可对其群体数量进行间接定量.这种方法具有选择性强、灵敏度高、稳定而又经济的优点,对于跟踪和回收释放至环境中的靶细菌具有重要的应用价值.

    Abstract:

    A luminescence measurement of the luxAB-genes-marked strain (Pseudomonas fluoreseens X16L2) was carried out in liquid culture and soil microcosms.The curves of luminescence kinetics of X16L2 in the liquid culture and soils were similar.The time reaching stable luminescence was about 7 nun after the luciferase substrate (n-decanal) was added.The results also showed that the bioluminescence could reflect the biomass of X16L2 in liquid culture,and the light output of X16L2 was closely related to not only the number.of viable cells but also the cell physiological activity.Soil conditions and native microorganisms had great effects on the survival of the introduced strain,including the number of viable cells and light output as well as the potential luminescence of X16L2.This study also demonstrated that luminometry could not only in situ detect the physiological activity of lux-genes-marked strain in the samples,but also measure its population indirectly.This method was a rapid and economical technique with high stability and sensitivity,and strong selectivity for tracking and recovering target microorganisms released to the environments.

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王平,王绩,胡正嘉,李阜棣.发光酶基因标记荧光假单胞菌X16L2的发光研究[J].土壤学报,1998,35(4):545-552. DOI:10.11766/trxb199705300414 Wang Ping, Wang Ji, Hu Zheng-jia, Li Fu-di. BIOLUMINESCENCE OF LUXAB-GENES-MARKED PSEUDOMONAS FLUORESCENS X16L2[J]. Acta Pedologica Sinica,1998,35(4):545-552.

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  • 收稿日期:1997-05-30
  • 最后修改日期:1997-12-05
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  • 在线发布日期: 2013-02-25
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