Titel: Mikrobiell diagnostik med PCR blir kliniskt värdefull när analystiden kortas [summary] 2004 nr 17 sid 1488-92

Läs/ladda hem artikeln: Översikt Artikeln i pdf-format (utskriftskvalitet) Sid 1488 Sid 1489 Sid 1490 Sid 1491 Sid 1492 Om Läkartidningens fulltext på Internet Hämta Acrobat Reader

Ämnesord:
Polymeraskedjereaktion
Tidsfaktorer
Diagnos
Bakteriella infektioner
Virussjukdomar
















Sök liknande artiklar (ny funktion på försök)

Summary:
PCR was introduced in 1985 by Mullis and was immediately recognized as a valuable tool in biomedical research and was awarded the Nobel Prize in 1993. Two culture-negative meningitis cases are described where Haemophilus influenzae and Neisseria meningitidis were found by 16SRNA-PCR. The modern real time PCR technology using fluorescent probes (hybridization probes, lightup probes, molecular beacons etc) for detection of the PCR-product or on DNA microarray chips, is under development for routine use. Multiplex technology can be used to simultaneously detect multiple microorganisms as well as resistance genes. Using super-convection with ultracentrifugation high-speed PCR, results can be obtained in 10 minutes and the amplificate can also be analyzed by DNA-sequencing to achieve species identification as well as detection of resistance gene mutations. The technique has mainly been applied to viruses, but is now slowly adapted to bacteria, fungi, protozoa and helminths. PCR is especially well suited for slow growing bacteria like Mycobacteria, fastidious organisms like Bartonella and contagious agents like tularemia, but also for malaria and fungi, where the advantages in sensitivity and speed can be exploited. The limit for application to routine analysis will depend on the development of simple and fast procedures for nucleic acid extraction, as well as interpretation of the PCR analysis per se, since highly efficient thermocyclers now are on the markets.
Jan Fohlman, Jonas Blomberg, Gunnar Fröman, Lars Engstrand, Anders Johansson, Göran Friman
Läkartidningen 2004;101:1488-92
Correspondence: Jan Fohlman, infektionskliniken, Akademiska sjukhuset, SE-751 85 Uppsala, Sweden
(jan.fohlman@ltkronoberg.se; jan.fohlman@academic.se)