Method for automated extraction and purification of nucleic acids and its implementation in microfluidic system
A method and a microfluidic device for automated extraction and purification of nucleic acids from biological samples have been developed. The method involves disruption of bacterial cells and/or viral particles by combining enzymatic and chemical lysis procedures followed by solid-phase sorbent ext...
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Veröffentlicht in: | Applied biochemistry and microbiology 2011-03, Vol.47 (2), p.211-220 |
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creator | Mamaev, D. D. Khodakov, D. A. Dementieva, E. I. Filatov, I. V. Yurasov, D. A. Cherepanov, A. I. Vasiliskov, V. A. Smoldovskaya, O. V. Zimenkov, D. V. Gryadunov, D. A. Mikhailovich, V. M. Zasedatelev, A. S. |
description | A method and a microfluidic device for automated extraction and purification of nucleic acids from biological samples have been developed. The method involves disruption of bacterial cells and/or viral particles by combining enzymatic and chemical lysis procedures followed by solid-phase sorbent extraction and purification of nucleic acids. The procedure is carried out in an automated mode in a microfluidic module isolated from the outside environment, which minimizes contact of the researcher with potentially infectious samples and, consequently, decreases the risk of laboratory-acquired infections. The module includes reservoirs with lyophilized components for lysis and washing buffers; a microcolumn with a solid-phase sorbent; reservoirs containing water, ethanol, and water-ethanol mixtures for dissolving freeze-dried buffer components, washing the microcolumn, and eluting of nucleic acids; and microchannels and valves needed for directing fluids inside the module. The microfluidic module is placed into the control unit that delivers pressure, executes heating, mixing of reagents, and movement of solutions within the microfluidic module. The microfluidic system performs extraction and purification of nucleic acids with high efficiency in 40 min, and nucleic acids extracted can be directly used in PCR reaction and microarray assays. |
doi_str_mv | 10.1134/S0003683811020128 |
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D. ; Khodakov, D. A. ; Dementieva, E. I. ; Filatov, I. V. ; Yurasov, D. A. ; Cherepanov, A. I. ; Vasiliskov, V. A. ; Smoldovskaya, O. V. ; Zimenkov, D. V. ; Gryadunov, D. A. ; Mikhailovich, V. M. ; Zasedatelev, A. S.</creator><creatorcontrib>Mamaev, D. D. ; Khodakov, D. A. ; Dementieva, E. I. ; Filatov, I. V. ; Yurasov, D. A. ; Cherepanov, A. I. ; Vasiliskov, V. A. ; Smoldovskaya, O. V. ; Zimenkov, D. V. ; Gryadunov, D. A. ; Mikhailovich, V. M. ; Zasedatelev, A. S.</creatorcontrib><description>A method and a microfluidic device for automated extraction and purification of nucleic acids from biological samples have been developed. The method involves disruption of bacterial cells and/or viral particles by combining enzymatic and chemical lysis procedures followed by solid-phase sorbent extraction and purification of nucleic acids. The procedure is carried out in an automated mode in a microfluidic module isolated from the outside environment, which minimizes contact of the researcher with potentially infectious samples and, consequently, decreases the risk of laboratory-acquired infections. The module includes reservoirs with lyophilized components for lysis and washing buffers; a microcolumn with a solid-phase sorbent; reservoirs containing water, ethanol, and water-ethanol mixtures for dissolving freeze-dried buffer components, washing the microcolumn, and eluting of nucleic acids; and microchannels and valves needed for directing fluids inside the module. The microfluidic module is placed into the control unit that delivers pressure, executes heating, mixing of reagents, and movement of solutions within the microfluidic module. 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The method involves disruption of bacterial cells and/or viral particles by combining enzymatic and chemical lysis procedures followed by solid-phase sorbent extraction and purification of nucleic acids. The procedure is carried out in an automated mode in a microfluidic module isolated from the outside environment, which minimizes contact of the researcher with potentially infectious samples and, consequently, decreases the risk of laboratory-acquired infections. The module includes reservoirs with lyophilized components for lysis and washing buffers; a microcolumn with a solid-phase sorbent; reservoirs containing water, ethanol, and water-ethanol mixtures for dissolving freeze-dried buffer components, washing the microcolumn, and eluting of nucleic acids; and microchannels and valves needed for directing fluids inside the module. 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The microfluidic system performs extraction and purification of nucleic acids with high efficiency in 40 min, and nucleic acids extracted can be directly used in PCR reaction and microarray assays.</description><subject>Automation</subject><subject>Biochemistry</subject><subject>Biological samples</subject><subject>Biomedical and Life Sciences</subject><subject>Biophysics</subject><subject>Enzymes</subject><subject>Ethanol</subject><subject>Life Sciences</subject><subject>Medical Microbiology</subject><subject>Microbiology</subject><subject>Nucleic acids</subject><subject>Reagents</subject><issn>0003-6838</issn><issn>1608-3024</issn><fulltext>true</fulltext><rsrctype>article</rsrctype><creationdate>2011</creationdate><recordtype>article</recordtype><sourceid>ABUWG</sourceid><sourceid>AFKRA</sourceid><sourceid>AZQEC</sourceid><sourceid>BENPR</sourceid><sourceid>CCPQU</sourceid><sourceid>DWQXO</sourceid><sourceid>GNUQQ</sourceid><recordid>eNp1kctKBDEQRYMoOI5-gLvgxlVrHv1IljL4ghEX6rrJJBXN0N0ZkzQ4f2_GFgTFVXGrzr1UUQidUnJBKS8vnwghvBZcUEoYoUzsoRmtiSg4YeU-mu3GxW5-iI5iXGcpayFnyD9AevMGWx-wGpPvVQKD4SMFpZPzA1aDwZsxOOu0-mp4i4dRd-A0VtqZ-EW4FLHrNx30MKSJcwPunQ7edqMzGY7bmKA_RgdWdRFOvuscvdxcPy_uiuXj7f3ialloXjap4FZqWUFdNnWlFSUNFcbWIGi10qJmTSNJBWVjjCqF5Q2nsiIGJKw0g6wJn6PzKXcT_PsIMbW9ixq6Tg3gx9iKhlEmiZCZPPtFrv0YhrxcK6pKknKKoxOUD4oxgG03wfUqbFtK2t0D2j8PyB42eWJmh1cIP8H_mz4B9R6IcQ</recordid><startdate>20110301</startdate><enddate>20110301</enddate><creator>Mamaev, D. 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D.</au><au>Khodakov, D. A.</au><au>Dementieva, E. I.</au><au>Filatov, I. V.</au><au>Yurasov, D. A.</au><au>Cherepanov, A. I.</au><au>Vasiliskov, V. A.</au><au>Smoldovskaya, O. V.</au><au>Zimenkov, D. V.</au><au>Gryadunov, D. A.</au><au>Mikhailovich, V. M.</au><au>Zasedatelev, A. S.</au><format>journal</format><genre>article</genre><ristype>JOUR</ristype><atitle>Method for automated extraction and purification of nucleic acids and its implementation in microfluidic system</atitle><jtitle>Applied biochemistry and microbiology</jtitle><stitle>Appl Biochem Microbiol</stitle><date>2011-03-01</date><risdate>2011</risdate><volume>47</volume><issue>2</issue><spage>211</spage><epage>220</epage><pages>211-220</pages><issn>0003-6838</issn><eissn>1608-3024</eissn><abstract>A method and a microfluidic device for automated extraction and purification of nucleic acids from biological samples have been developed. The method involves disruption of bacterial cells and/or viral particles by combining enzymatic and chemical lysis procedures followed by solid-phase sorbent extraction and purification of nucleic acids. The procedure is carried out in an automated mode in a microfluidic module isolated from the outside environment, which minimizes contact of the researcher with potentially infectious samples and, consequently, decreases the risk of laboratory-acquired infections. The module includes reservoirs with lyophilized components for lysis and washing buffers; a microcolumn with a solid-phase sorbent; reservoirs containing water, ethanol, and water-ethanol mixtures for dissolving freeze-dried buffer components, washing the microcolumn, and eluting of nucleic acids; and microchannels and valves needed for directing fluids inside the module. The microfluidic module is placed into the control unit that delivers pressure, executes heating, mixing of reagents, and movement of solutions within the microfluidic module. The microfluidic system performs extraction and purification of nucleic acids with high efficiency in 40 min, and nucleic acids extracted can be directly used in PCR reaction and microarray assays.</abstract><cop>Dordrecht</cop><pub>SP MAIK Nauka/Interperiodica</pub><doi>10.1134/S0003683811020128</doi><tpages>10</tpages></addata></record> |
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subjects | Automation Biochemistry Biological samples Biomedical and Life Sciences Biophysics Enzymes Ethanol Life Sciences Medical Microbiology Microbiology Nucleic acids Reagents |
title | Method for automated extraction and purification of nucleic acids and its implementation in microfluidic system |
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