Real-time DNA microarrays: reality check

Chagovetz, Alexander M.; Blair, Steve

doi:10.1042/bst0370471

Cited by 23 publications

(19 citation statements)

References 57 publications

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“…The effects of this variability are exacerbated when results from different labo-ratories are compared, making it essential to consider appropriate quality assurance measures (18 ). Disregard of technical issues is not confined to RT-qPCR: unreliable quantification and false-positive results are also observed with microarrays (19,20 ), and estimating relative transcript abundance by next generation sequencing is inconsistent not just at low levels of coverage but even when coverage levels are high (21 ).…”

confidence: 99%

Variability of the Reverse Transcription Step: Practical Implications

et al. 2015

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confidence: 99%

Variability of the Reverse Transcription Step: Practical Implications

et al. 2015

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“…The increase of DNA in each cycle is proportional to hybridization of probes, which in turn is proportional to the increase in the emitted fluorescence. The use of probes allows identifying polymorphisms and mutations; however, these are more complex and expensive than intercalating agents [35,36,37]. …”

Section: Real Time Pcrmentioning

confidence: 99%

Polymerase Chain Reaction: Types, Utilities and Limitations

Hernández-Rodríguez¹,

Ramírez²

2012

Polymerase Chain Reaction

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“…DNA Polymerase enzyme assist the synthesis of deoxyribonucleic acid from deoxynucleotide substrates on a fiber deoxyribonucleic acid templet. deoxyribonucleic acid enzyme adds nucleotides to the 3` finishes of oligonucleotide once it's toughened to an extended templet deoxyribonucleic acid 5 . It contains an area complementary to the oligonucleotide.…”

Section: Basic Principle Of Pcrmentioning

confidence: 99%

Polymerase Chain Reaction and Its Clinical Application: A Review

Tomar¹

2018

J. Pharm. Sci. Innov.

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Polymerase chain reaction is a popular method in molecular diagnostic in which small amount of DNA undergo five steps of denaturation, primer attachment, again repeating to form number of copies, in analogous way continued round of amplification many identical copies can be produced. There are numerous factors which play significant role in this technique like denaturation temperature (94°C), Annealing temperature (40 to 60°C), Extension temperature (72°C) also with type of DNA polymerase enzyme use like natural (Taq) or recombinant (Amplitaq). All polymerase varies in term of their properties (Their thermostability, exonuclease activity, extension rate, reverse transcriptase activity, molecular weight, resulting DNA end and so on). Its applicability is very wide ranging from genetic fingerprinting, forensic investigation, cloning, mutation detection, microarray. It is still in its development phase new advances are made every day, still need to overcome some of its drawback like variation in parameters, starting material quantification.

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Real-time DNA microarrays: reality check

Cited by 23 publications

References 57 publications

Variability of the Reverse Transcription Step: Practical Implications

Variability of the Reverse Transcription Step: Practical Implications

Polymerase Chain Reaction: Types, Utilities and Limitations

Polymerase Chain Reaction and Its Clinical Application: A Review

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