Restriction fragment length polymorphism: Difference between revisions

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Line 1: {{Short description\|Molecular biology technique}} In [[molecular biology]], '''restriction fragment length polymorphism''' ('''RFLP''') is a technique that exploits variations in [[homology (biology)\|homologous]] [[DNA]] sequences, known as [[~~polymorphism~~Gene ~~(biology)~~polymorphism\|polymorphisms]], ~~in order to distinguish individuals,~~ populations, or species or to pinpoint the locations of [[gene]]s within a sequence. The term may refer to a polymorphism itself, as detected through the differing locations of [[restriction site\|restriction enzyme sites]], or to a related laboratory technique by which such differences can be illustrated. In '''RFLP analysis''', a DNA sample is digested into fragments by one or more [[restriction enzyme]]s, and the resulting ''restriction fragments'' are then separated by [[gel electrophoresis]] according to their size. ~~Although~~RFLP analysis is now largely obsolete due to the emergence of inexpensive [[DNA sequencing]] technologies, ~~RFLP~~but ~~analysis~~it was the first [[DNA profiling]] technique inexpensive enough to see widespread application. RFLP analysis was an important early tool in [[genome mapping]], localization of genes for [[genetic disorder]]s, determination of [[Genetic testing\|risk]] for disease, and [[DNA paternity testing\|paternity testing]]. ==RFLP analysis== The basic technique for the detection of RFLPs ~~involves~~ fragmenting a sample of DNA with the application of a [[restriction enzyme]], which can selectively cleave a DNA molecule wherever a short, [[recognition sequence\|specific]] [[nucleic acid sequence\|sequence]] is recognized in a process known as a [[restriction digest]]. The DNA fragments produced by the digest are then separated by length through a process known as [[agarose gel electrophoresis]] and transferred to a membrane via the [[Southern blot]] procedure. [[Nucleic acid hybridization\|Hybridization]] of the membrane to a labeled [[Hybridization probe\|DNA probe]] then determines the length of the fragments which are [[Complementarity (molecular biology)\|complementary]] to the probe. A restriction fragment length polymorphism is said to occur when the length of a detected fragment varies between individuals, indicating non-identical sequence homologies. Each fragment length is considered an [[allele]], whether it actually contains a [[coding DNA\|coding region]] or not, and can be used in subsequent genetic analysis. [[File:RFLPDemo1.gif\|right\|thumb\|450px\|Schematic for RFLP by cleavage site loss]] [[File:RFLP genotyping.gif\|right\|thumb\|360px\|Analysis and inheritance of allelic RFLP fragments (NIH)]] Line 26 ⟶ 27: The technique for RFLP analysis is, however, slow and cumbersome. It requires a large amount of sample DNA, and the combined process of probe labeling, DNA fragmentation, electrophoresis, blotting, hybridization, washing, and [[autoradiography]] can take up to a month to complete. A limited version of the RFLP method that used [[Oligomer restriction\|oligonucleotide probes]] was reported in 1985.<ref name="SaikiScharf1985">{{cite journal\|last1=Saiki\|first1=R.\|last2=Scharf\|first2=S\|last3=Faloona\|first3=F\|last4=Mullis\|first4=K.\|last5=Horn\|first5=G.\|last6=Erlich\|first6=H.\|last7=Arnheim\|first7=N\|title=Enzymatic amplification of beta-globin genomic sequences and restriction site analysis for diagnosis of sickle cell anemia\|journal=Science\|volume=230\|issue=4732\|year=1985\|pages=1350–1354\|issn=0036-8075\|doi=10.1126/science.2999980\|pmid=2999980\|bibcode=1985Sci...230.1350S}}</ref> The results of the [[Human Genome Project]] have largely replaced the need for RFLP mapping, and the identification of many [[single-nucleotide polymorphism]]s (SNPs) in that project (as well as the direct identification of many disease genes and mutations) has replaced the need for RFLP disease linkage analysis (see [[SNP genotyping]]). The analysis of VNTR alleles continues, but is now usually performed by [[polymerase chain reaction]] (PCR) methods. For example, the standard [[National DNA database\|protocols]] for [[DNA fingerprinting]] involve PCR analysis of [[CODIS\|panels]] of more than a dozen VNTRs. RFLP is still used in marker-assisted selection. Terminal restriction fragment length polymorphism (TRFLP or sometimes T-RFLP) is a technique initially developed for characterizing bacterial communities in mixed-species samples. The technique has also been applied to other groups including soil fungi. TRFLP works by PCR amplification of DNA using primer pairs that have been labeled with fluorescent tags. The PCR products are then digested using RFLP enzymes and the resulting patterns visualized using a DNA sequencer. The results are analyzed either by simply counting and comparing bands or peaks in the TRFLP profile, or by matching bands from one or more TRFLP runs to a database of known species. ~~The~~A ~~technique~~number isof ~~similar~~different insoftware ~~some~~tools ~~aspects~~have been developed to ~~[[temperature~~automate ~~gradient~~the ~~gel~~process of band matching, comparison and data basing of TRFLP profiles.<ref>{{Cite journal ~~electrophoresis~~\|~~temperature~~last1=Heras ~~gradient]]~~\|first1=J. or\|last2=Dominguez ~~[[denaturing~~\|first2=C. ~~gradient~~\|last3=Mata ~~gel~~\|first3=E. ~~electrophoresis]]~~\|last4=Pascual ~~(TGGE~~\|first4=V. ~~and~~\|last5=Lozano ~~DGGE)~~\|first5=C. \|last6=Torres \|first6=C. \|last7=Zarazaga \|first7=M. \|date=2015-03-29 \|title=A survey of tools for analysing DNA fingerprints \|url=https://academic.oup.com/bib/article-lookup/doi/10.1093/bib/bbv016 \|journal=Briefings in Bioinformatics \|volume=17 \|issue=6 \|language=en \|pages=903–911 \|doi=10.1093/bib/bbv016 \|pmid=25825453 \|issn=1467-5463}}</ref> The technique is similar in some aspects to [[temperature gradient gel electrophoresis\|temperature gradient]] or [[denaturing gradient gel electrophoresis]] (TGGE and DGGE). The sequence changes directly involved with an RFLP can also be analyzed more quickly by PCR. Amplification can be directed across the altered restriction site, and the products digested with the restriction enzyme. This method has been called [[Cleaved Amplified Polymorphic Sequence]] (CAPS). Alternatively, the amplified segment can be analyzed by [[allele-specific oligonucleotide]] (ASO) probes, a process that can often be done by a simple [[dot blot]]. Line 42 ⟶ 45: ==External links== *[https://www.ncbi.nlm.nih.gov~~/projects/genome~~/probe/~~doc~~docs/~~TechRFLP~~techrflp/ nih.~~shtml~~gov] {{molecular genetics methods}} {{DEFAULTSORT:Restriction Fragment Length Polymorphism}} [[Category:Biochemistry detection methods]] [[Category:Genomics techniques]]▼ [[Category:Molecular biology]] ▲[[Category:Genomics]]