{"title":"荧光染料转移的流式细胞术定量测定间隙连接细胞间通讯。","authors":"M H Juul, E Rivedal, T Stokke, T Sanner","doi":"10.3109/15419060009040307","DOIUrl":null,"url":null,"abstract":"<p><p>Gap junction intercellular communication (GJIC) is involved in several aspects of normal cell behaviour, and disturbances in this type of communication have been associated with many pathological conditions. Reliable and accurate methods for the determination of GJIC are therefore important in studies of cell biology. (Tomasetto, C., Neveu, M.J., Daley, J., Horan, P.K. and Sager, R. (1993) Journal of Cell Biology, 122, 157-167) reported some years ago the use of flow cytometer to determine transfer between cells of a mobile dye, calcein, as a measure of cell communication through gap junctions. In spite of this being a method with potential for quantitative and reliable determination of GJIC, it has been modestly used, possibly due to technical difficulties. In the present work we have illustrated several ways to use flow cytometric data to express cell communication through gap junctions. The recipient cells were pre-stained with the permanent lipophilic dye PKH26, and the donor cell population were loaded with the gap junction permeable dye, calcein. We show that the method may be used to measure the effect of chemicals on GJIC, and that the information is reliable, objective and reproducible due to the large number of cells studied. The data may give additional information to that obtained with other methods, since the effect observed will be on the establishment of cell communication as compared to what is observed for microinjection or scrape loading, where the effect is on already established communication. This is probably the reason for the more potent effects of DMSO on GJIC measured by the present method than on already existing GJIC measured by microinjection or quantitative scrape loading. We also show that the problem related to the mobile dye calcein not being fixable with aldehydes will not affect the results as long as the cells are kept on ice in the dark and analysed by flow cytometer within the first hours after formalin cell fixation.</p>","PeriodicalId":79325,"journal":{"name":"Cell adhesion and communication","volume":"7 6","pages":"501-12"},"PeriodicalIF":0.0000,"publicationDate":"2000-01-01","publicationTypes":"Journal Article","fieldsOfStudy":null,"isOpenAccess":false,"openAccessPdf":"https://sci-hub-pdf.com/10.3109/15419060009040307","citationCount":"15","resultStr":"{\"title\":\"Quantitative determination of gap junction intercellular communication using flow cytometric measurement of fluorescent dye transfer.\",\"authors\":\"M H Juul, E Rivedal, T Stokke, T Sanner\",\"doi\":\"10.3109/15419060009040307\",\"DOIUrl\":null,\"url\":null,\"abstract\":\"<p><p>Gap junction intercellular communication (GJIC) is involved in several aspects of normal cell behaviour, and disturbances in this type of communication have been associated with many pathological conditions. Reliable and accurate methods for the determination of GJIC are therefore important in studies of cell biology. (Tomasetto, C., Neveu, M.J., Daley, J., Horan, P.K. and Sager, R. (1993) Journal of Cell Biology, 122, 157-167) reported some years ago the use of flow cytometer to determine transfer between cells of a mobile dye, calcein, as a measure of cell communication through gap junctions. In spite of this being a method with potential for quantitative and reliable determination of GJIC, it has been modestly used, possibly due to technical difficulties. In the present work we have illustrated several ways to use flow cytometric data to express cell communication through gap junctions. The recipient cells were pre-stained with the permanent lipophilic dye PKH26, and the donor cell population were loaded with the gap junction permeable dye, calcein. We show that the method may be used to measure the effect of chemicals on GJIC, and that the information is reliable, objective and reproducible due to the large number of cells studied. The data may give additional information to that obtained with other methods, since the effect observed will be on the establishment of cell communication as compared to what is observed for microinjection or scrape loading, where the effect is on already established communication. This is probably the reason for the more potent effects of DMSO on GJIC measured by the present method than on already existing GJIC measured by microinjection or quantitative scrape loading. 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引用次数: 15
摘要
间隙连接细胞间通讯(GJIC)参与了正常细胞行为的几个方面,这种通讯的干扰与许多病理状况有关。因此,可靠和准确的测定GJIC的方法在细胞生物学研究中非常重要。(Tomasetto, C., Neveu, m.j., Daley, J., Horan, P.K. and Sager, R. (1993) Journal of Cell Biology, 122, 157-167)几年前报道使用流式细胞仪测定一种可移动染料钙黄蛋白在细胞间的转移,作为通过间隙连接的细胞通信的测量。尽管这是一种有可能定量和可靠地测定GJIC的方法,但可能由于技术上的困难,它的使用并不多。在目前的工作中,我们已经说明了几种使用流式细胞术数据通过间隙连接表达细胞通信的方法。受体细胞用永久性亲脂性染料PKH26预染色,供体细胞群用间隙连接渗透性染料钙黄蛋白负载。我们表明,该方法可用于测量化学物质对GJIC的影响,并且由于研究的细胞数量多,信息可靠,客观,可重复性好。这些数据可以提供其他方法所获得的额外信息,因为与显微注射或刮擦加载所观察到的效果相比,所观察到的效果将是对细胞通信的建立,而显微注射或刮擦加载的效果是对已经建立的通信的影响。这可能是DMSO对本方法测量的GJIC的影响比已经存在的显微注射或定量刮擦加载测量的GJIC更有效的原因。我们还表明,只要在福尔马林细胞固定后的第一个小时内将细胞放在冰上,在黑暗中用流式细胞仪分析,与移动染料钙黄蛋白不能用醛固定有关的问题不会影响结果。
Quantitative determination of gap junction intercellular communication using flow cytometric measurement of fluorescent dye transfer.
Gap junction intercellular communication (GJIC) is involved in several aspects of normal cell behaviour, and disturbances in this type of communication have been associated with many pathological conditions. Reliable and accurate methods for the determination of GJIC are therefore important in studies of cell biology. (Tomasetto, C., Neveu, M.J., Daley, J., Horan, P.K. and Sager, R. (1993) Journal of Cell Biology, 122, 157-167) reported some years ago the use of flow cytometer to determine transfer between cells of a mobile dye, calcein, as a measure of cell communication through gap junctions. In spite of this being a method with potential for quantitative and reliable determination of GJIC, it has been modestly used, possibly due to technical difficulties. In the present work we have illustrated several ways to use flow cytometric data to express cell communication through gap junctions. The recipient cells were pre-stained with the permanent lipophilic dye PKH26, and the donor cell population were loaded with the gap junction permeable dye, calcein. We show that the method may be used to measure the effect of chemicals on GJIC, and that the information is reliable, objective and reproducible due to the large number of cells studied. The data may give additional information to that obtained with other methods, since the effect observed will be on the establishment of cell communication as compared to what is observed for microinjection or scrape loading, where the effect is on already established communication. This is probably the reason for the more potent effects of DMSO on GJIC measured by the present method than on already existing GJIC measured by microinjection or quantitative scrape loading. We also show that the problem related to the mobile dye calcein not being fixable with aldehydes will not affect the results as long as the cells are kept on ice in the dark and analysed by flow cytometer within the first hours after formalin cell fixation.
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