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TheNativeAntigenCompany/Canine Parvovirus 2 VP2 Capsid Protein/100ug/REC31788-100

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货号:REC31788-100
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品牌:TheNativeAntigenCompany
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REC31788_SDS-PAGE

SDS-PAGE: Image shows purified recombinant VP2 protein.

REC31788_EM

Electron Micrographs: Images show CPV virus like particles produced by expression of the recombinant VP2 protein.

CANINE PARVOVIRUS 2 VP2 CAPSID PROTEIN

Canine Parvovirus 2 VP2 capsid protein is a recombinant protein, cloned and expressed in insect cells. It can be used as a calibrator in immunoassays for detection of CPV or as an antigen in CPV antibody titer analyses. The protein is also able to assemble into virus‑like particles.

PRODUCT DETAILS – CANINE PARVOVIRUS 2 VP2 CAPSID PROTEIN

  • Canine Parvovirus 2 VP2 capsid protein.
  • Manufactured in insect cells with greater than 90% purity as determined by SDS-PAGE.
  • Protein is derived from CPV Type 2b and consists of 584 amino acid residues. Does not contain any affinity tags.
  • Can be used as calibrator or standard in immunoassays for CPV immunodetection or antigen in immunoassays for determination of CPV antibody titre in canine blood.
  • Immunoreactivity is confirmed by reaction with our monoclonal antibodies (MAB12400 – MAB12404), specific to canine parvovirus.

BACKGROUND

Canine parvovirus (CPV) Canine parvovirus type 2 (CPV‑2) causes severe and highly contagious disease in dogs. CPV-2 is a non-enveloped single-stranded DNA virus in the Parvoviridae family, 20-26 nm in diameter with an icosahedral symmetry. It is a relatively new virus that was first recognized in 1978 and then spread worldwide in only 1-2 years (Carmichael, 2005). CPV is highly contagious and is transmitted by the faecal-oral route through contact with faeces from infected dogs or contaminated surfaces. It is the most important enteric virus infecting canids.

CPV‑2 has a non‑enveloped spherical capsid assembled from three proteins (VP1, VP2 and VP3). Capsid protein self-assembles to form an icosahedral capsid with a T=1 symmetry, about 22 nm in diameter, and consisting of 60 copies of a combination of VP1 (5‑6 copies) and VP2 (54‑55 copies). VP1 and VP2 are products of the same gene that are generated by alternative splicing of viral mRNA but VP1 has an additional 143aa in its N‑terminus compared to VP2. Empty capsids can be assembled from VP2 alone. VP3 is present only in full virions and is formed as the result of proteolytic cleavage of 19aa from the N‑terminus of VP2. The capsid encapsulates the genomic ssDNA and capsid proteins are responsible for the attachment to a host cell receptor. Phylogenetic analysis showed that all CPVs derived from a single common ancestor, and CPV-2 likely arose when it acquired mutations that allowed binding to the canine transferrin receptor (TfR) type-1. TfR plays a key role in the susceptibility of cells to infection by parvoviruses (reviewed in Miranda & Thompson, 2016). This attachment induces virion internalization predominantly through clathrin-endocytosis. Binding to the host receptors also induces capsid rearrangements leading to surface exposure of VP1 phospholipase A2-like region and nuclear localization signal(s). VP1 N-terminus might serve as a lipolytic enzyme to breach the endosomal membrane during entry into host cell. Intracytoplasmic transport involves microtubules and interaction between capsid proteins and host dynein. Exposure of nuclear localization signal may allow nuclear import of capsids.

The main method for controlling the disease in domestic animals is by vaccination. However, given the viruses ability for rapid evolution, the continued development of vaccines is likely to be an important area of research (reviewed in Miranda & Thompson, 2016).

This VP2 protein and corresponding antibodies have been manufactured specifically for Canine Parvovirus immunoassay development.

REFERENCES

  • Carmichael L (2005). An annotated historical account of canine parvovirus. J. Vet. Med. B Infect. Dis. Vet. Public Health. 52 (7–8): 303–11.
  • Miranda & Thompson (2016). Canine parvovirus: the worldwide occurrence of antigenic variants. J Gen Virol. 97(9):2043-2057.
  • Shackelton et al. (2005). High rate of viral evolution associated with the emergence of carnivore parvovirus. Proc. Natl. Acad. Sci. USA. 102 (2): 379–384.

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TheNativeAntigenCompany我们在测定开发方面拥有多年经验。根据具体应用,我们建议并测试多种不同的ELISA格式,从简单的直接ELISA到具有封闭抗原的间接ELISA和双抗原结合ELISA。您不仅可以从我们的高级测定开发科学家那里获得咨询的好处,而且我们的内部表达系统还可以用于生产天然折叠的和完全糖基化的蛋白质和抗体,以用作最高质量的独特试剂,从而使您的ELISA处于优势反对竞争。我们的能力包括:+   ELISA设计和格式咨询+   定制抗原和抗体生产+   使用定制抗原作为免疫原(mAbs和pAbs)产生抗体+   ELISA中的抗原/抗体对优化+   与酶结合以检测抗体+   板涂+   ELISA优化  我们可以在项目的任何阶段为您的ELISA分析的开发提供支持,  提供定制服务,这些灵活性可以评估用于分析的最佳抗体  对,直至商业套件的全面开发。 如果您的概念还处于早期阶段,那么我们可以准备您的抗原,  提高您的抗体,并使用它们来开发特定的ELISA分析以满足您的需求。