DNA primer - definitie. Wat is DNA primer
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Wat (wie) is DNA primer - definitie

SHORT STRAND OF RNA OR DNA THAT SERVES AS A STARTING POINT FOR DNA SYNTHESIS
RNA primer; Primer RNA; Degenerate primer; RNA primers; Rna primer; PCR-Primer; PCR Primer; Primer (genetics); DNA primer; PCR primer; Primer Design; Primer (dna); Primer removal; Universal primer; Universal primers; DNA primers
  • PCR]]

Trap primer         
PLUMBING DEVICE OR VALVE THAT ADDS WATER TO TRAPS
Trap seal primer
A trap primer (or trap seal primer) is a plumbing device or valve that adds water to traps. The water seals in traps are needed to prevent sewer gases from entering buildings, but because this water is exposed to the air, it is subject to evaporation over time in infrequently used floor drains, leading to the release of sewer gas into the environment.
Primer with Various Instructions         
BOOK BY PETAR BERON
Fish Primer
Primer with Various Instructions (, Bukvar s razlichni poucheniya), better known as the Fish Primer (, Riben bukvar, original spelling: Боукварь съ различны пооученіѧ), was a Bulgarian schoolbook, the first primer (and first book) printed in modern Bulgarian. It is considered by an author to be the first Bulgarian encyclopedia.
DNA glycosylase         
  • 
Hydrolysis of cytosine to uracil
ENZYMES INVOLVED IN BASE EXCISION REPAIR
GO system; Dna glycosylases; Dna glycosylase; DNA glycosylases; Dna Glycosylase
DNA glycosylases are a family of enzymes involved in base excision repair, classified under EC number EC 3.2.

Wikipedia

Primer (molecular biology)

A primer is a short single-stranded nucleic acid used by all living organisms in the initiation of DNA synthesis. DNA polymerase (responsible for DNA replication) enzymes are only capable of adding nucleotides to the 3’-end of an existing nucleic acid, requiring a primer be bound to the template before DNA polymerase can begin a complementary strand. DNA polymerase adds nucleotides after binding to the RNA primer and synthesizes the whole strand. Later, the RNA strands must be removed accurately and replace them with DNA nucleotides forming a gap region known as a nick that is filled in using an enzyme called ligase. The removal process of the RNA primer requires several enzymes, such as Fen1, Lig1, and others that work in coordination with DNA polymerase, to ensure the removal of the RNA nucleotides and the addition of DNA nucleotides. Living organisms use solely RNA primers, while laboratory techniques in biochemistry and molecular biology that require in vitro DNA synthesis (such as DNA sequencing and polymerase chain reaction) usually use DNA primers, since they are more temperature stable. Primers can be designed in laboratory for specific reactions such as polymerase chain reaction (PCR). When designing PCR primers, there are specific measures that must be taken into consideration, like the melting temperature of the primers and the annealing temperature of the reaction itself. Moreover, the DNA binding sequence of the primer in vitro has to be specifically chosen, which is done using a method called basic local alignment search tool (BLAST) that scans the DNA and finds specific and unique regions for the primer to bind.