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Rabbit anti-Vesicular stomatitis Indiana virus L Polyclonal Antibody, HRP conjugated

The antibody against L was raised in rabbit using the Recombinant Vesicular stomatitis Indiana virus RNA-directed RNA polymerase L protein (598-784AA) as the immunogen. This antibody exists as a hrp conjugated isotype IgG, purified by protein G with a purity greater than 95%. This antibody has been validated on ELISA.

ADC-02553A

The antibody against L was raised in rabbit using the Recombinant Vesicular stomatitis Indiana virus RNA-directed RNA polymerase L protein (598-784AA) as the immunogen. This antibody exists as a hrp conjugated isotype IgG, purified by protein G with a purity greater than 95%. This antibody has been validated on ELISA.

$299.00

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Specifications


Cat.No ADC-02553A ClonalityPolyclonal
Host SpeciesRabbitTarget NameL
FormLiquidSpecies ReactivityVesicular stomatitis Indiana virus
IsotypeIgGStorage Buffer0.01M PBS, 0.03% Proclin 300; Constituents: 50% Glycerol, PH 7.4
Purification Method>95%, Protein G purifiedConjugateHRP conjugated
ApplicationELISAStorageUpon receipt

Immunogen Information


Immunogen DescriptionRecombinant Vesicular stomatitis Indiana virus RNA-directed RNA polymerase L protein (598-784AA)Target SpeciesVesicular stomatitis Indiana virus
Immunogen SequenceComplete sequences for the immunogen, target protein, and peptides are available upon request.Uniprot IDQ8B0H0
Background Information
  • Uniprot Id

    Q8B0H0

  • Target Species

    Vesicular stomatitis Indiana virus

  • Target Name

    L

  • Target Function

    Responsible for RNA synthesis (replicase and transcriptase), cap addition, and cap methylation. Performs also the polyadenylation of subgenomic mRNAs by a stuttering mechanism at a slipery stop site present at the end of viral genes. The template is composed of the viral RNA tightly encapsidated by the nucleoprotein (N). The viral polymerase binds to the genomic RNA at the 3' leader promoter, thereby initiating either genome replication or mRNA transcription. In the transcription mode, the polymerase performs the sequential transcription of all mRNAs using a termination-reinitiation mechanism responding to gene start and gene end signals. Some polymerase disengage from the template at each gene junction, resulting in a decreasing abundance of transcripts from the 3' to the 5' end of the genome. The first gene is the most transcribed, and the last the least transcribed. The viral phosphoprotein helps the polymerase to engage the N-RNA template and acts as processivity factor. Polyribonucleotidyl transferase (PRNTase) adds the cap structure when the nascent RNA chain length has reached few nucleotides. Ribose 2'-O methylation of viral mRNA cap precedes and facilitates subsequent guanine-N-7 methylation, both activities being carried by the viral polymerase. In the replication mode, the polymerase replicates the whole viral genome without recognizing the gene end transcriptional signals. The ability of the polymerase to override the gene end signals as it is producing the antigenome is probably due to replicative RNA becoming encapsidated with nucleoprotein as it is synthesized.

  • Target Subcellular Location

    Virion. Host cytoplasm.

  • Target Protein Families

    Rhabdoviridae protein L family

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