Tesi sul tema "Polymerase chain reaction"
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Feugeas, Olivier. "Pcr (polymerase chain reaction) et vih". Lille 2, 1990. http://www.theses.fr/1990LIL2M264.
Testo completoLantz, Pär-G. "PCR-based detection of microorganisms in complex biological samples". Lund : Dept. of Applied Microbiology, Lund University, 1998. http://catalog.hathitrust.org/api/volumes/oclc/39178906.html.
Testo completoVerhaegen, Monique Elise. "Novel approaches in quantitative polymerase chain reaction". Thesis, National Library of Canada = Bibliothèque nationale du Canada, 1998. http://www.collectionscanada.ca/obj/s4/f2/dsk1/tape10/PQDD_0021/MQ52489.pdf.
Testo completoChiou, Jeffrey Tsungshuan. "A novel capillary polymerase chain reaction machine". Thesis, Massachusetts Institute of Technology, 2001. http://hdl.handle.net/1721.1/8864.
Testo completoIncludes bibliographical references (p. 254-268).
I built a novel prototype capillary polymerase chain reaction machine. The purpose was to perform a single reaction as fast as possible with a reaction volume - 100 nl. The PCR mix is in the form of a 1 /1 droplet that moves between three heat zones inside of a 1 mm I.D. capillary filled with mineral oil via pneumatic actuation. A laser beam waveguides down the capillary until it strikes the drop, at which point it scatters. The scatter is picked up by a series of photodiodes to provide position feedback. Due to the efficient heat transfer arrangement, the drop can transition between different temperature steps in -2 seconds, which includes both drop motion and temperature equilibration. It was extensively tested in both 10-cycle and 30-cycle PCR, including nearly 200 successful 30-cycle runs. The 30-cycle PCR was typically 74% (as high as 78%) efficient, and took only 23 minutes. This compares well with existing machines in the literature.
by Jeffrey Tsungshuan Chiou.
Ph.D.
Clackson, Timothy Piers. "Antibody engineering using the polymerase chain reaction". Thesis, University of Cambridge, 1991. http://ethos.bl.uk/OrderDetails.do?uin=uk.bl.ethos.316695.
Testo completoLinley, M. "The detection of polymerase inhibiting lesions using the polymerase arrest polymerase chain reaction assay". Thesis, Swansea University, 2004. http://ethos.bl.uk/OrderDetails.do?uin=uk.bl.ethos.637924.
Testo completoNebbali, M. "Human gene mapping using the polymerase chain reaction". Thesis, University of Nottingham, 1992. http://ethos.bl.uk/OrderDetails.do?uin=uk.bl.ethos.317395.
Testo completoBorges, Pinto Lais Izabel. "Alu-polymerase chain reaction genomic fingerprinting in neuroblastoma". Thesis, University of Newcastle Upon Tyne, 2001. http://ethos.bl.uk/OrderDetails.do?uin=uk.bl.ethos.366679.
Testo completoErill, Sagalés Ivan. "High-speed Polymerase chain reaction in CMOS-compatible chips". Doctoral thesis, Universitat Autònoma de Barcelona, 2002. http://hdl.handle.net/10803/3031.
Testo completoEn el transcurso de esta tesis doctoral, se ha llevado a cabo el desarrollo un proceso tecnológico común para la fabricación de DNA-chips multifunción (i.e. sistemas versátiles basados en PCR y electroforesis), poniendo un especial énfasis en la compatibilidad con los procesos CMOS estándar, a fin de conseguir desarrollar prototipos proto-industriales. Como demostrador de esta puesta a punto tecnológica, se han diseñado, fabricado y testado chips de PCR, y la PCR en chips ha sido optimizada con respecto a materiales de fabricación, metodologías de inserción/extracción, composición bioquímica de la mix de PCR, diferentes configuraciones de calentadores/sensores (Peltier/termopares vs. resistencias integradas) y la cinética de la reacción.
In the last decade of the twentieth century, the fields of µ-TAS and, more specifically, DNA-chips have acquired increasing importance in the microsystems arena. The main reason for this surge of interest lies in the advantages these new devices seek to bring forth: faster, cheaper and completely automated analyses, and also in the outbreak of novel analytical techniques (e.g. hybridization chips). In the particular case of DNA-chips, functional prototypes have been demonstrated for PCR, LCR, gel electrophoresis, di-electrophoresis, hybridization and various combinations of these techniques, whilst hybridization chips (mainly arrayer chips) have become a successful market application. But, even though a considerable amount of work has been carried out in these few years, much research is still required to address fundamental problems of DNA-chips.
In this doctoral work, a common-ground technological setup for the production of multifunction DNA-chips (i.e. PCR plus electrophoresis systems) has been laid down, placing strong emphasis in its compatibility with standard CMOS processes in order to produce proto-industrial prototypes. As a demonstrator of this technological setup, PCR-chips have been designed, manufactured and tested, and the chip PCR reaction has been optimized with respect to surface materials, insertion and extraction methods, biochemical mix composition, heater/sensor setups (Peltier/thermocouple vs. thin-film driven systems) and reaction kinetics.
Aydin, Gamze. "Detection Of Genetically Modified Maize Via Polymerase Chain Reaction". Master's thesis, METU, 2004. http://etd.lib.metu.edu.tr/upload/3/12605495/index.pdf.
Testo completoBallagi-Pordány, András. "Application of polymerase chain reaction (PCR) in veterinary virology /". Uppsala : Sveriges lantbruksuniv, 1995. http://epsilon.slu.se/avh/1995/91-576-4997-9.gif.
Testo completoWoolford, Alison Jane. "Use of polymerase chain reaction for detection of mycobacteria". Thesis, University of Surrey, 1995. http://ethos.bl.uk/OrderDetails.do?uin=uk.bl.ethos.308497.
Testo completoGurram, Neil (Neil K. ). "A mathematical model of polymerase chain reaction induced stutter". Thesis, Massachusetts Institute of Technology, 2016. http://hdl.handle.net/1721.1/106012.
Testo completoThis electronic version was submitted by the student author. The certified thesis is available in the Institute Archives and Special Collections.
Cataloged from student-submitted PDF version of thesis.
Includes bibliographical references (page 48).
This is a thesis on understanding stutter present in capillary electropherogram readouts as this methodology forms the basis of current DNA fingerprinting. The readouts come from taking samples of various initial template masses of DNA from different individuals, applying polymerase chain reaction (PCR) to the samples, and then running the amplified copies through capillary electrophoresis to produce a readout of peak heights corresponding to alleles on various loci. The alleles correspond to the number of repeats of microsatellites that are usually two to six base pairs in length called short tandem repeats (STRs); the number of repeats of various STRs defines a person's DNA fingerprint. This process introduces artifacts in measurement. Of particular interest in this thesis is stutter, the phenomenon where amplicons with fewer or greater number of STR repeats than the true allele count are generated as an artifact of the PCR. It is of interest to understand the source and nature for this stutter distribution for small starting masses, as it has ramifications on the ability to accurately determine a match between a DNA sample and a crime scene sample. Understanding the stutter distribution in this thesis is achieved through data analysis, probabilistic modeling, and statistics. We find that a mathematical model that combines stochastic effects from PCR with fluorescent noise explains the most significant features of the observed phenomena.
by Neil Gurram.
M. Eng.
Lewis, Monte. "Thermal cycling design alternatives for the polymerase chain reaction". College Park, Md. : University of Maryland, 2005. http://hdl.handle.net/1903/3061.
Testo completoThesis research directed by: Dept. of Mechanical Engineering. Title from t.p. of PDF. Includes bibliographical references. Published by UMI Dissertation Services, Ann Arbor, Mich. Also available in paper.
Way, Jaw-Shiow Chu. "Specific detection of Salmonella by multiplex polymerase chain reaction". Diss., The University of Arizona, 1993. http://hdl.handle.net/10150/186207.
Testo completoSikorsky, Jan A. "Effect of DNA base modification on polymerase chain reaction efficiency and fidelity". Huntington, WV : [Marshall University Libraries], 2005. http://www.marshall.edu/etd/descript.asp?ref=554.
Testo completoMuwonge, Abubaker. "Detection Of Genetically Modified Potatoes By The Polymerase Chain Reaction". Master's thesis, METU, 2005. http://etd.lib.metu.edu.tr/upload/12605783/index.pdf.
Testo completoWhite, Adam. "Development and application of microfluidic single-cell polymerase chain reaction". Thesis, University of British Columbia, 2015. http://hdl.handle.net/2429/55734.
Testo completoScience, Faculty of
Graduate
Tsang, Tsui-ying Stella, e 曾璀瑩. "Application of quantitative polymerase chain reaction in the diagnosisof thalassaemia". Thesis, The University of Hong Kong (Pokfulam, Hong Kong), 2006. http://hub.hku.hk/bib/B45010948.
Testo completoGamma, Torres Rafael Enrique. "Application of polymerase chain reaction to rhinovirus detection and analysis". Thesis, University of Essex, 1992. http://ethos.bl.uk/OrderDetails.do?uin=uk.bl.ethos.293589.
Testo completoKoc, Yasemin. "Optimization of continuous flow polymerase chain reaction with microfluidic reactors". Thesis, Imperial College London, 2008. http://hdl.handle.net/10044/1/8184.
Testo completoAllmann, Michael. "Applications of the polymerase chain reaction (PCR) in food chemistry /". [S.l.] : [s.n.], 1994. http://www.ub.unibe.ch/content/bibliotheken_sammlungen/sondersammlungen/dissen_bestellformular/index_ger.html.
Testo completoMello, Richard. "IDENTIFICATION OF DQ ALPHA POLYMORPHISM USING THE POLYMERASE CHAIN REACTION". VCU Scholars Compass, 1991. https://scholarscompass.vcu.edu/etd/5213.
Testo completoTsang, Tsui-ying Stella. "Application of quantitative polymerase chain reaction in the diagnosis of thalassaemia /". View the Table of Contents & Abstract, 2006. http://sunzi.lib.hku.hk/hkuto/record/B36433895.
Testo completoTsui, Wai-yan. "Determination of PTEN mutations in prostate cancer in Chinese". Hong Kong : University of Hong Kong, 2001. http://sunzi.lib.hku.hk/hkuto/record.jsp?B23736173.
Testo completo顔鴻儀 e Hung-yee Ngan. "Molecular diagnosis of penicilliosis marneffei". Thesis, The University of Hong Kong (Pokfulam, Hong Kong), 2001. http://hub.hku.hk/bib/B31970035.
Testo completoBasten, Graham Paul. "Induction of phase II enzymes by isothiocyanates : an investigation using quantitative RT-PCR". Thesis, University of East Anglia, 2002. http://ethos.bl.uk/OrderDetails.do?uin=uk.bl.ethos.393316.
Testo completoNgan, Hung-yee. "Molecular diagnosis of penicilliosis marneffei". Hong Kong : University of Hong Kong, 2001. http://sunzi.lib.hku.hk/hkuto/record.jsp?B23595978.
Testo completoMcMullen, Kevin Patrick. "Inhibitory effects of food matrices on real-time reverse transcription polymerase chain reaction detection of foodborne viruses". [Tampa, Fla. : s.n.], 2003. http://purl.fcla.edu/fcla/etd/SFE0000100.
Testo completoSonmezalp, C. Zeynep. "Detection Of Genetically Modified Insect Resistant Tomato Via Polymerase Chain Reaction". Master's thesis, METU, 2004. http://etd.lib.metu.edu.tr/upload/3/12605493/index.pdf.
Testo completoDuman, Zeynep. "Polymerase Chain Reaction (pcr) For Detection Of Borrelia Burgdorferi Sensu Lato". Master's thesis, METU, 2008. http://etd.lib.metu.edu.tr/upload/2/12609199/index.pdf.
Testo completoRos, Bascuñana Carlos. "Diagnostic application of the polymerase chain reaction (PCR) in veterinary microbiology /". Uppsala : Swedish Univ. of Agricultural Sciences (Sveriges lantbruksuniv.), 1997. http://epsilon.slu.se/avh/1997/91-576-5247-3.gif.
Testo completoWalker, Ken R. "Rapid detection of Listeria monocytogenes in salad by polymerase chain reaction". Auburn, Ala, 2005. http://repo.lib.auburn.edu/2005%20Summer/master's/WALKER_KEN_28.pdf.
Testo completoPhaneuf, Christopher. "Infrared laser-mediated polymerase chain reaction in a polymer microfluidic device". Diss., Georgia Institute of Technology, 2014. http://hdl.handle.net/1853/53068.
Testo completoTully, Gillian. "DNA profiling for forensic identification : evaluation of polymerase chain reaction methods". Thesis, Cardiff University, 1996. http://ethos.bl.uk/OrderDetails.do?uin=uk.bl.ethos.264882.
Testo completoDiss, Timothy Charles. "The polymerase chain reaction in the characterisation and diagnosis of lymphomas". Thesis, University College London (University of London), 1996. http://ethos.bl.uk/OrderDetails.do?uin=uk.bl.ethos.338653.
Testo completoOrganji, Sameer R. A. "Detection of #Beta#-lactam resistant Streptococcus pneumoniae by polymerase chain reaction". Thesis, University of Bristol, 1998. http://ethos.bl.uk/OrderDetails.do?uin=uk.bl.ethos.297824.
Testo completoSim, Steven Poh Chuen. "An integrated chip-based device for droplet-flow polymerase chain reaction". Thesis, Imperial College London, 2016. http://hdl.handle.net/10044/1/56111.
Testo completoLiao, Yu-Hua. "Polymerase chain reaction based cloning of acetate kinase in propionibacterium acidipropionici". The Ohio State University, 2004. http://rave.ohiolink.edu/etdc/view?acc_num=osu1072778140.
Testo completoHolladay, Ervin Blair. "Viral gene detection in oral neoplasms using the polymerase chain reaction". The Ohio State University, 1991. http://rave.ohiolink.edu/etdc/view?acc_num=osu1345129906.
Testo completoHolladay, E. Blair. "Viral gene detection in oral neoplasms using the polymerase chain reaction /". The Ohio State University, 1991. http://rave.ohiolink.edu/etdc/view?acc_num=osu1487694702781994.
Testo completoLiao, Yu-Hua. "Polymerase chain reaction based cloning of acetate kinase in Propionibacterium acidipropionici /". Connect to this title online, 2003. http://rave.ohiolink.edu/etdc/view?acc%5Fnum=osu1072778140.
Testo completoLiu, Tingting. "Electrokinetic Real-Time Polymerase Chain Reaction Toward Point-Of-Care Diagnosis". Diss., The University of Arizona, 2015. http://hdl.handle.net/10150/579083.
Testo completoSu, Ying-Tu, e 蘇英圖. "Application of MicroEmusification:Emulsion Polymerase Chain Reaction". Thesis, 2009. http://ndltd.ncl.edu.tw/handle/51940901593932821213.
Testo completo國立臺灣海洋大學
機械與機電工程學系
97
In this thesis, soft lithography technique was used to produce a micro emulsion chip. This chip can handle tiny volume of DNA solution for polymerase chain reation (ePCR). The DNA solution is dispersed in the emulsified droplets in a continuous oil phase, and the droplets become reaction space for PCR. As a result, the consistency of the multiple types of DNA templates existing in the original reaction space can be improved by emulsification process. Also, it will reduce competitive sequence interference and improve DNA magnification. Differing from usual micro emulsification chips, this study focuses on the technical problems involved in dealing with tiny and expensive DNA solution in order to avoid non-uniform droplets in the transient of droplet generation. The main ideas are as follows: (1) Let water first go through transient process and produce water droplets; (2) Use water and bubble to place DNA solution in between, and pass it through emulsification hydrodynamic focusing channel; (3) Use pneumatic membrane valves control the stop and flow of water and DNAsolution. Characterization of the emulsification chips includes droplet sizes, uniformity of droplets and hot-resistance of water-in-oil droplets. The smallest droplet diameter is less than 10 μm and the coefficient of variation is about 2%. The resulting electrophoretograms of both single or multiple templates’ PCR demonstrate that ePCR can improve the precision of amplified DNA segments. It is suggested from the experiment results that ePCR was proven to be efficient and could be used in further genetic research Key word: ePCR, DNA template, transient process, tiny-volume micro-emulsification
Gi, Kao Li, e 高麗姬. "ABO Genotyping for Mutiplex Polymerase Chain Reaction". Thesis, 1999. http://ndltd.ncl.edu.tw/handle/82466547226309854097.
Testo completo中央警察大學
刑事警察研究所
87
Abstract ABO blood group is clinically the most important blood group system in transfusion medicine including fours common different phenotypes . It has been a valuable tool in transfusion medicine , physical anthropology , disputed parentage testing , human identification , and in forensic analysis . Historically , forensic and clinical labatories utilize serological techniques to identify ABO blood type . The testing of forensic samples for ABO types using serological techniques has several drawbacks . We has simplified the identification of ABO types by taking advantage of previouly reported ABO DNA sequence difference . The use of single strand conformation polymorphism(SSCP)can separate sequence polymorphism than differ by only one base . We has investigated in 260 Chinese donors by multiplexed Polymerase Chain Reaction . In this study the ABO alleles from exon 6 , producing a 212/213 bp fragment , and exon 7, which produces a fragment of 272 bp , were separated by non-denaturing polyacrylamide gels . The two exons were amplified in a single reaction that produces similar quantities of DNA for both exons . However , in 260 SSCP patterens we can clustered 9 into different distinct and discernible groups . A concordance rate of 98.5 ﹪(256/260 samples)observed between the actural genotype and the serologically-based predicted genotype . These results indicate that the assay provides a rapid , accurate , and simple method for ABO genotyping that serves as a useful supplement to standard serological ABO typing .
Chen, Jhao-Rong, e 陳昭榮. "Micro Rayleigh-Bénard polymerase chain reaction system". Thesis, 2005. http://ndltd.ncl.edu.tw/handle/05888212591754965876.
Testo completo國立清華大學
工程與系統科學系
93
Polymerase chain reaction (PCR) is a molecular biological method for the in vitro amplification of nucleic acid molecule. In this thesis, the research object was to design a micro PCR system which involved a Rayleigh-Bénard convection PCR chip, measurement circuits, and temperature control circuits. Rayleigh-Bénard convection PCR chip was easy to be fabricated, and the sample solution in it can transit its temperature immediately. Thus, the faster the speed of flow is, the higher heating and cooling rate is. Rayleigh-Bénard convection PCR chip can be divided into two parts. First part is a chip with micro heaters and micro temperature sensors. Second part is PDMS reaction chamber designed by Rayleigh-Bénard convection theory. Temperature control system is designed to keep temperature on the top and bottom chips by Pulse width modulation control. Analog temperature signal is precisely measured by circuits. Then the signal is processed by an 8051 single chip, and the output power of micro heaters is controlled to adjust the temperature of top and down plates. Finally, agarose gel electrophoresis is used to verify the practicability of Rayleigh-Bénard convection PCR system. By comparing with the PCR experiments done by the commercial PCR machine and our chips, our chips can plenty decrease the reaction time. And By comparing with the simulation and PCR experiments of different designed sizes, users can use setted parameters and CFD results to do optimal designs and then decrease the total reaction time in the future.
Tao, Yo-Shen, e 刁宥升. "Design Of Polymerase Chain Reaction System Controller". Thesis, 2002. http://ndltd.ncl.edu.tw/handle/76827215729605694932.
Testo completo國立暨南國際大學
電機工程學系
90
DNA analysis is a crucial process for biotechnology. Polymerase chain reaction (PCR) is an imperative step for performing DNA analysis. PCR can proliferate a small quantity of DNA sample to a large quantity enough for DNA analysis in a short time. Our goal is to develop a PCR system chip by integrating standard CMOS process and MEMS process. In this thesis, an 8-bit 4-level pipelined programmable micro-controller for temperature control during PCR process is designed by HDL description and implemented by using field programmable gate array (FPGA). The micro-controller includes modules of data path and control unit. Verilog hardware description language is used to model the modules. The individual module is functionally verified by Max Plus II of Altera and integrated into an 8-bit micro-controller. The micro-controller is realized by a FPGA chip, and then micro program for the temperature control of PCR is downloaded into the ROM in FPGA for system test. The micro-controller proposed in this thesis is very simple and easy to implement. It is suitable for general low speed applications. In order to easily integrate the micro-controller into other applications, we will try to parameterize its design variables for adjusting its hardware structure in future works.
Gao, Li-Ji, e 高麗姬. "ABO Genotyping for Multiplex Polymerase Chain Reaction". Thesis, 1998. http://ndltd.ncl.edu.tw/handle/7433nn.
Testo completo中央警察大學
刑事警察研究所
87
ABO blood group is clinically the most important blood group system in transfusion medicine including fours common different phenotypes . It has been a valuable tool in transfusion medicine , physical anthropology , disputed parentage testing , human identification , and in forensic analysis . Historically , forensic and clinical labatories utilize serological techniques to identify ABO blood type . The testing of forensic samples for ABO types using serological techniques has several drawbacks . We has simplified the identification of ABO types by taking advantage ofpreviouly reported ABO DNA sequence difference . The use of single strand conformation polymorphism ( SSCP ) can separate sequence polymorphism than differ by only one base . We has investigated in 260 Chinese donors by multiplexed Polymerase Chain Reaction . In this study the ABO alleles from exon 6 , producing a 212/213 bp fragment , and exon 7, which produces a fragment of 272 bp, were separated by non-denaturing polyacrylamide gels. The two exons were amplified in a single reaction that produces similar quantities of DNA for both exons . However , in 260 SSCP patterens we can clustered 9 into different distinct and discernible groups . A concordance rate of 98.5 % (256/260 samples) observed between the actural genotype and the serologically-based predicted genotype . These results indicate that the assay provides a rapid , accurate , and simple method for ABO genotyping that serves as a useful supplement to standard serological ABO typing.
Lin, Min-Han. "PDMS (polydimethylsiloxane) Based Polymerase Chain Reaction Component Design". 2005. http://www.cetd.com.tw/ec/thesisdetail.aspx?etdun=U0001-2707200515463700.
Testo completo張澔任. "Detection of Chlamydophila abortus by polymerase chain reaction". Thesis, 2000. http://ndltd.ncl.edu.tw/handle/59334353234665564833.
Testo completo國立中興大學
獸醫微生物學研究所
88
The purpose of this study was to develop a specific polymerase chain reaction for rapid detection of Chlamydophila abortus. We selected the published chlamydial omp A and 16S-23S rRNA gene sequences from GeneBank, and respectively aligned these sequences to find suitable regions for Chlamydophila abortus-specific primer design. The alignment of 16S-23S rRNA gene sequences revealed no suitable region for primer design, while the alignment of omp A gene sequences revealed many suitable regions for Chlamydophila abortus- specific primer design. We designed several primer pairs from these suitable regions of omp A gene by Primer_3, and finally we selected 358f-868r, 433f-834r, 835f-1064r and 402f-1064r four primer pairs for the examination of detection of Chlamydophila abortus by polymerase chain reaction. The result showed that all the four primer pairs were specific for Chlamydophila abortus, so that our polymerase chain reaction with these primer pairs could permit the rapid and specific detedtion of Chlamydophila abortus, and the 358f-868r primer pair was the most sensitive pair. By this study we have developed a specific polymerase chain reaction for rapid detection of Chlamydophila abortus.