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AB320051

HIV1 p24 ELISA Kit- Extracellular

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HIV1 p24 ELISA Kit- Extracellular is a single-wash 90-min Simplestep used to quantify HIV1 p24 with a sensitivity of 4.3 pg/ml. The assay uses a simple mix-wash-read protocol with just one incubation and one wash step.

- Colorimetric Sandwich ELISA - 450 nm readout : works on any standard plate reader
- Different formats for different needs: 10x96 plates for bulk orders and 384-well plate for higher throughput

View Alternative Names

Gag-Pol polyprotein, Pr160Gag-Pol, gag-pol

9 Images
Sandwich ELISA - HIV1 p24 ELISA Kit- Extracellular (AB320051)
  • sELISA

Supplier Data

Sandwich ELISA - HIV1 p24 ELISA Kit- Extracellular (AB320051)

Recombinant p24 was spiked into the following samples, treated with Cell Extraction Buffer SSW and diluted in a 2-fold dilution series in Sample Diluent NSW. Samples (prior to the treatment) are 100% HEK-293 cell culture supernatant and monkey serum. The interpolated dilution factor corrected values are plotted (mean +/- SD, n=2).

Sandwich ELISA - HIV1 p24 ELISA Kit- Extracellular (AB320051)
  • sELISA

Supplier Data

Sandwich ELISA - HIV1 p24 ELISA Kit- Extracellular (AB320051)

WHO/NIBSC international reference reagent 90/636 (native p24 protein isolated from detergent treated HIV1) was spiked into the following samples, treated with Cell Extraction Buffer SSW and diluted in a 2-fold dilution series in Sample Diluent NSW. Samples (prior to the treatment) are 100% human serum, human plasma (heparin), HEK-293 cell culture supernatant, and monkey serum. The interpolated dilution factor corrected values are plotted (mean +/- SD, n=2).

Sandwich ELISA - HIV1 p24 ELISA Kit- Extracellular (AB320051)
  • sELISA

Supplier Data

Sandwich ELISA - HIV1 p24 ELISA Kit- Extracellular (AB320051)

Standard curve comparison between HIV1 p24 SimpleStep ELISA kit (ab320051) and traditional ELISA kit from leading competitor. SimpleStep ELISA kit shows comparable sensitivity.

Sandwich ELISA - HIV1 p24 ELISA Kit- Extracellular (AB320051)
  • sELISA

Supplier Data

Sandwich ELISA - HIV1 p24 ELISA Kit- Extracellular (AB320051)

Recombinant p24 was spiked into the following human samples, treated with Cell Extraction Buffer SSW and diluted in a 2-fold dilution series in Sample Diluent NSW. Samples (prior to the treatment) are 100% serum, plasma (citrate), plasma (EDTA), and plasma (heparin). The interpolated dilution factor corrected values are plotted (mean +/- SD, n=2).

Sandwich ELISA - HIV1 p24 ELISA Kit- Extracellular (AB320051)
  • sELISA

Supplier Data

Sandwich ELISA - HIV1 p24 ELISA Kit- Extracellular (AB320051)

Serial dilutions of HIV1 p24 (group M subtype B, strain 92418), HIV1 p24 (group M subtype B, strain HXB2), HIV1 p24 (group M subtype B, isolate NY5), HIV1 p24 (group O, strain BCF06), and HIV1 p24 (group M, subtype C, strain 92BR025) were prepared within the working range of the assay and assayed for reactivity. Raw O.D. values (mean +/- SD) are graphed. This kit does not react with recombinant HIV1 p24 from group M, subtype C, strain 92BR025.

Sandwich ELISA - HIV1 p24 ELISA Kit- Extracellular (AB320051)
  • sELISA

Supplier Data

Sandwich ELISA - HIV1 p24 ELISA Kit- Extracellular (AB320051)

Example of HIV1 p24 standard curve. Background-subtracted data values (mean +/- SD) are graphed.

Sandwich ELISA - HIV1 p24 ELISA Kit- Extracellular (AB320051)
  • sELISA

Supplier Data

Sandwich ELISA - HIV1 p24 ELISA Kit- Extracellular (AB320051)

Standard curve comparison between HIV1 p24 SimpleStep ELISA kit (ab320051) and traditional ELISA kit from leading competitor. SimpleStep ELISA kit shows comparable sensitivity.

Sandwich ELISA - HIV1 p24 ELISA Kit- Extracellular (AB320051)
  • sELISA

Supplier Data

Sandwich ELISA - HIV1 p24 ELISA Kit- Extracellular (AB320051)

Example of HIV1 p24 standard curve in 96-well vs. 384-well plate. Background-subtracted data values (mean +/- SD) are graphed.

Sandwich ELISA - HIV1 p24 ELISA Kit- Extracellular (AB320051)
  • sELISA

Supplier Data

Sandwich ELISA - HIV1 p24 ELISA Kit- Extracellular (AB320051)

Recombinant p24 was spiked into the following human samples, treated with Cell Extraction Buffer SSW and diluted in a 2-fold dilution series in Sample Diluent NSW in 96-well vs. 384-well plates. Samples (prior to the treatment) are 100% human serum. The interpolated dilution factor corrected values are plotted (mean +/- SD, n=2).

Key facts

Detection method

Colorimetric

Sample types

Serum, Citrate plasma, EDTA Plasma, Heparin Plasma, Cell culture supernatant

Reacts with

Human immunodeficiency virus

Assay type

Sandwich (quantitative)

Sensitivity

= 4.3 pg/mL

Range

15.625 - 1000 pg/mL

Assay time

1h 30m

Assay Platform

Pre-coated microplate (12 x 8 well strips)

Reactivity data

{ "title": "Reactivity Data", "filters": { "stats": ["", "Reactivity", "Dilution Info", "Notes"] }, "values": { "sELISA": { "reactivity":"TESTED_AND_REACTS", "dilution-info":"", "notes":"<p></p>" } } }

Product details

HIV1 p24 SimpleStep ELISA® kit is a single-wash 90 min sandwich ELISA designed for the quantitative measurement of HIV1 p24 protein in Serum, Cit plasma, EDTA Plasma, Hep Plasma, and Cell culture supernatant. Quantitate  HIV1 p24 with 4.3 pg/ml sensitivity.

SimpleStep ELISA® technology employs capture antibodies conjugated to an affinity tag that is recognized by the monoclonal antibody used to coat our SimpleStep ELISA® plates. This approach to sandwich ELISA allows the formation of the antibody-analyte sandwich complex in a single step, significantly reducing assay time. See the SimpleStep ELISA® protocol summary in the image section for further details. Our SimpleStep ELISA® technology provides several benefits:

-Single-wash protocol reduces assay time to 90 minutes or less
-High sensitivity, specificity and reproducibility from superior antibodies
-Fully validated in biological samples
-96-wells plate breakable into 12 x 8 wells strips, available in 10-pack (10 x 96-well plates)
-Also available in a fully validated 384-well format.

Precision

[ { "reproducibilityType": "Intra", "sample": "Supernatant", "replicates": 8, "mean": null, "standardDeviation": null, "coefficientOfVariability": "5.1" }, { "reproducibilityType": "Inter", "sample": "Supernatant", "replicates": 3, "mean": null, "standardDeviation": null, "coefficientOfVariability": "7.8" } ]

Recovery

[ { "sample": "Serum", "range": "86 - 97 %", "average": "= 90" }, { "sample": "Citrate plasma", "range": "84 - 98 %", "average": "= 90" }, { "sample": "EDTA Plasma", "range": "82 - 96 %", "average": "= 89" }, { "sample": "Heparin Plasma", "range": "91 - 102 %", "average": "= 96" }, { "sample": "Cell culture supernatant", "range": "91 - 103 %", "average": "= 95" } ]

What's included?

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Properties and storage information

Shipped at conditions
Blue Ice
Appropriate short-term storage conditions
+4°C
Appropriate long-term storage conditions
+4°C
Storage information
+4°C

Supplementary information

This supplementary information is collated from multiple sources and compiled automatically.

HIV1 p24 also known as HIV p24 protein is a core protein of the Human Immunodeficiency Virus type 1 (HIV-1). The p24 protein has a molecular weight of about 24 kDa. HIV1 p24 comprises part of the viral capsid which encases the viral RNA genome. This protein is prominently expressed during the early stages of HIV infection. The presence of HIV1 p24 is commonly detected through various laboratory techniques including the use of p24 ELISA kits.
Biological function summary

HIV1 p24 plays an important role in the viral life cycle. It assists in the formation and stability of the viral capsid which is critical for maintaining the integrity of the viral core. HIV p24 is not a lone actor; it is part of the structural framework and interacts with other viral proteins to facilitate the viral assembly and maturation processes. The detection of HIV1 p24 is a marker for viral replication and infection stage.

Pathways

The function of HIV1 p24 aligns significantly within the HIV replication pathway and the host’s immune response pathway. HIV p24 is intrinsically tied to processes of viral assembly alongside proteins like Gag and Pol coordinating to ensure successful viral replication. Furthermore the immune system recognizes the HIV1 p24 protein thereby integrating it into the host immune response which is important in disease progression and for diagnostic purposes like in the HIV ELISA assay.

HIV1 p24 is integrally connected to HIV/AIDS a disorder that profoundly affects the immune system. The presence of HIV p24 in the bloodstream is an early marker of infection and is frequently monitored to track the disease's progression. Alterations in the levels of p24 protein relate to the efficiency of therapeutic interventions. The study of HIV1 p24 also brings focus on its interaction with the CD4 receptor which is pivotal in the viral entry process further linking various stages of the HIV infection cycle to potential therapeutic targets.

Product protocols

Target data

Gag-Pol polyprotein. Mediates, with Gag polyprotein, the essential events in virion assembly, including binding the plasma membrane, making the protein-protein interactions necessary to create spherical particles, recruiting the viral Env proteins, and packaging the genomic RNA via direct interactions with the RNA packaging sequence (Psi). Gag-Pol polyprotein may regulate its own translation, by the binding genomic RNA in the 5'-UTR. At low concentration, the polyprotein would promote translation, whereas at high concentration, the polyprotein would encapsidate genomic RNA and then shut off translation.. Matrix protein p17. Targets the polyprotein to the plasma membrane via a multipartite membrane-binding signal, that includes its myristoylated N-terminus (By similarity). Matrix protein is part of the pre-integration complex. Implicated in the release from host cell mediated by Vpu. Binds to RNA (By similarity).. Capsid protein p24. Forms the conical core that encapsulates the genomic RNA-nucleocapsid complex in the virion (PubMed : 8648689). Most core are conical, with only 7% tubular. The core is constituted by capsid protein hexamer subunits. The core is disassembled soon after virion entry (PubMed : 12660176). Host restriction factors such as monkey TRIM5-alpha or TRIMCyp bind retroviral capsids and cause premature capsid disassembly, leading to blocks in reverse transcription. Capsid restriction by TRIM5 is one of the factors which restricts HIV-1 to the human species (PubMed : 23785198). Host PIN1 apparently facilitates the virion uncoating (By similarity). On the other hand, interactions with PDZD8 or CYPA stabilize the capsid (PubMed : 24554657).. Nucleocapsid protein p7. Encapsulates and protects viral dimeric unspliced genomic RNA (gRNA). Binds these RNAs through its zinc fingers. Acts as a nucleic acid chaperone which is involved in rearangement of nucleic acid secondary structure during gRNA retrotranscription. Also facilitates template switch leading to recombination. As part of the polyprotein, participates in gRNA dimerization, packaging, tRNA incorporation and virion assembly.. Protease. Aspartyl protease that mediates proteolytic cleavages of Gag and Gag-Pol polyproteins during or shortly after the release of the virion from the plasma membrane (PubMed : 11932404, PubMed : 9573231). Cleavages take place as an ordered, step-wise cascade to yield mature proteins (PubMed : 11932404, PubMed : 9573231). This process is called maturation (PubMed : 11932404, PubMed : 9573231). Displays maximal activity during the budding process just prior to particle release from the cell (PubMed : 11932404, PubMed : 9573231). Also cleaves Nef and Vif, probably concomitantly with viral structural proteins on maturation of virus particles (PubMed : 7835426). Hydrolyzes host EIF4GI and PABP1 in order to shut off the capped cellular mRNA translation. The resulting inhibition of cellular protein synthesis serves to ensure maximal viral gene expression and to evade host immune response (PubMed : 12660176, PubMed : 19914170). Also mediates cleavage of host YTHDF3 (PubMed : 32053707). Mediates cleavage of host CARD8, thereby activating the CARD8 inflammasome, leading to the clearance of latent HIV-1 in patient CD4(+) T-cells after viral reactivation; in contrast, HIV-1 can evade CARD8-sensing when its protease remains inactive in infected cells prior to viral budding (PubMed : 33542150).. Reverse transcriptase/ribonuclease H. Multifunctional enzyme that converts the viral RNA genome into dsDNA in the cytoplasm, shortly after virus entry into the cell. This enzyme displays a DNA polymerase activity that can copy either DNA or RNA templates, and a ribonuclease H (RNase H) activity that cleaves the RNA strand of RNA-DNA heteroduplexes in a partially processive 3' to 5' endonucleasic mode. Conversion of viral genomic RNA into dsDNA requires many steps. A tRNA(3)-Lys binds to the primer-binding site (PBS) situated at the 5'-end of the viral RNA. RT uses the 3' end of the tRNA primer to perform a short round of RNA-dependent minus-strand DNA synthesis. The reading proceeds through the U5 region and ends after the repeated (R) region which is present at both ends of viral RNA. The portion of the RNA-DNA heteroduplex is digested by the RNase H, resulting in a ssDNA product attached to the tRNA primer. This ssDNA/tRNA hybridizes with the identical R region situated at the 3' end of viral RNA. This template exchange, known as minus-strand DNA strong stop transfer, can be either intra- or intermolecular. RT uses the 3' end of this newly synthesized short ssDNA to perform the RNA-dependent minus-strand DNA synthesis of the whole template. RNase H digests the RNA template except for two polypurine tracts (PPTs) situated at the 5'-end and near the center of the genome. It is not clear if both polymerase and RNase H activities are simultaneous. RNase H probably can proceed both in a polymerase-dependent (RNA cut into small fragments by the same RT performing DNA synthesis) and a polymerase-independent mode (cleavage of remaining RNA fragments by free RTs). Secondly, RT performs DNA-directed plus-strand DNA synthesis using the PPTs that have not been removed by RNase H as primers. PPTs and tRNA primers are then removed by RNase H. The 3' and 5' ssDNA PBS regions hybridize to form a circular dsDNA intermediate. Strand displacement synthesis by RT to the PBS and PPT ends produces a blunt ended, linear dsDNA copy of the viral genome that includes long terminal repeats (LTRs) at both ends.. Integrase. Catalyzes viral DNA integration into the host chromosome, by performing a series of DNA cutting and joining reactions. This enzyme activity takes place after virion entry into a cell and reverse transcription of the RNA genome in dsDNA. The first step in the integration process is 3' processing. This step requires a complex comprising the viral genome, matrix protein, Vpr and integrase. This complex is called the pre-integration complex (PIC). The integrase protein removes 2 nucleotides from each 3' end of the viral DNA, leaving recessed CA OH's at the 3' ends. In the second step, the PIC enters cell nucleus. This process is mediated through integrase and Vpr proteins, and allows the virus to infect a non dividing cell. This ability to enter the nucleus is specific of lentiviruses, other retroviruses cannot and rely on cell division to access cell chromosomes. In the third step, termed strand transfer, the integrase protein joins the previously processed 3' ends to the 5' ends of strands of target cellular DNA at the site of integration. The 5'-ends are produced by integrase-catalyzed staggered cuts, 5 bp apart. A Y-shaped, gapped, recombination intermediate results, with the 5'-ends of the viral DNA strands and the 3' ends of target DNA strands remaining unjoined, flanking a gap of 5 bp. The last step is viral DNA integration into host chromosome. This involves host DNA repair synthesis in which the 5 bp gaps between the unjoined strands are filled in and then ligated. Since this process occurs at both cuts flanking the HIV genome, a 5 bp duplication of host DNA is produced at the ends of HIV-1 integration. Alternatively, Integrase may catalyze the excision of viral DNA just after strand transfer, this is termed disintegration.
See full target information gag-pol

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