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Swine IFN alpha 1 (Yeast-derived Recombinant Protein) - 5 micrograms

RP0010S-005
$150.00
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Type I interferons comprise a vast and growing group of IFN proteins. Homologous molecules to type I IFNs are found in many species, including all mammals, and some have been identified in birds, reptiles, amphibians and fish species. The mammalian types are designated IFN-alpha, IFN-beta, IFN-kappa, IFN-delta, IFN-epsilon, IFN-tau, IFN-omega, and IFN-zeta (also known as limitin). They are mainly involved in innate immune response against viral infection.

Swine IFN alpha 1 (Yeast-derived Recombinant Protein) - 5 micrograms
Catalog No.:
RP0010S-005
Quantity:
5 ug
Source:
The Swine IFN alpha 1 recombinant protein was produced in yeast and therefore does not have endotoxin, is naturally folded, and post-translationally modified.
MW:
The Swine IFN alpha recombinant protein has a predicted molecular weight of 19.0 kDa.
Protein Sequence:
CDLPQTHSLA HTRALRLLAQ MRRISPFSCL DHRRDFGSPH EAFGGNQVQK AQAMALVHEM LQQTFQLFST EGSAAAWNES LLHQFCTGLD QQLRDLEACV MQGAGLEGTP LLEEDSILAV RKYFHRLTLY LQEKSYSPCA WEIVRAEVMR SFSSSRNLQD RLRKKE (166)
Country of Origin:
USA
Applications:
The swine IFN alpha 1 endotoxin-free recombinant protein can be used in cell culture, as a IFN alpha ELISA Standard, and as a Western Blot Control.

31577832

Evaluation of PRRSv specific, maternally derived and induced immune response in Ingelvac PRRSFLEX EU vaccinated piglets in the presence of maternally transferred immunity.

Kraft C, Hennies R, Dreckmann K, Noguera M, Rathkjen PH, Gassel M, Gereke M.

PLoS One. 2019 Oct 2;14(10):e0223060. doi: 10.1371/journal.pone.0223060. eCollection 2019.

Applications: Measurement of Swine IFN alpha in bronchial alveolar lavage fluid by ELISA

Abstract

In this study, we analyzed PRRS virus (PRRSvspecific lymphocyte function in piglets vaccinated with Ingelvac PRRSFLEX EU® at two and three weeks of age in the presence of homologous maternal immunity. Complete analysis of maternal immunity to PRRSv was evaluated postpartum, as well as passive transfer of antibodies and T cells to the piglet through colostrum intake and before and after challenge with a heterologous PRRSv at ten weeks of age. Maternal-derived antibodies were detected in piglets but declined quickly after weaning. However, vaccinated animals restored PRRSv-specific antibody levels by anamnestic response to vaccination. Cell analysis in colostrum and milk revealed presence of PRRSv-specific immune cells at suckling with higher concentrations found in colostrum than in milk. In addition, colostrum and milk contained PRRSv-specific IgA and IgG that may contribute to protection of newborn piglets. Despite the presence of PRRSv-specific Peripheral Blood Mononuclear cells (PBMCs) in colostrum and milk, no PRRSv-specific cells could be detected from blood of the piglets at one or two weeks of life. Nevertheless, cellular immunity was detectable in pre-challenged piglets up to 7 weeks after vaccination while the non-vaccinated control group showed no interferon (IFN) γ response to PRRSv stimulation. After challenge, all piglets developed a PRRSv-specific IFNγ-response, which was more robust at significantly higher levels in vaccinated animals compared to the primary response to PRRSv in non-vaccinated animals. Cytokine analysis in the lung lumen showed a reduction of pro-inflammatory responses to PRRSv challenge in vaccinated animals, especially reduced interferon (IFN) α levels. In conclusion, vaccination of maternally positive piglets at 2 and 3 weeks of age with Ingelvac PRRSFLEX EU induced a humoral and cellular immune response to PRRSv and provided protection against virulent, heterologous PRRSv challenge.


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