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pT324/pS327-C5a1 (phospho-Complement C5a Receptor 1 Antibody)

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  • 7TM0032A
  • 100 µl
  • Rabbit
Threonine324/serine327 (T324/S327) is a major phosphorylation site of the C5a1 receptor. The... more

Threonine324/serine327 (T324/S327) is a major phosphorylation site of the C5a1 receptor. The pT324/pS327-C5a1 antibody detects phosphorylation in response to high- and low-efficacy agonists but not after PKC activation. T324/S327 phosphorylation is a key regulator of C5a1 desensitization, β-arrestin recruitment and internalization. The pT324/pS327-C5a1 antibody can by used for detection of the subcellular location of phosphorylated C5a1 receptors by immunocytochemistry.

  Alternative Names C5a1, C5AR1, Complement C5a Receptor 1, C5a Anaphylatoxin... more

 

Alternative Names C5a1, C5AR1, Complement C5a Receptor 1, C5a Anaphylatoxin Chemotactic Receptor 1
IUPHAR Target ID  32
UniProt ID  P21730
Western Blot (WB)  1:1000
Immunocytochemistry (ICC) 1:200
Species Reactivity   Human
Host / Isotype Rabbit / IgG
Class Polyclonal
Immunogen A synthetic phosphopeptide derived from human C5a1 around the phosphorylation site of Thr324/Ser327
Form  Liquid
Purification Antigen affinity chromatography
Storage buffer Dulbecco's PBS, pH 7.4, with 150 mM NaCl, 0.02% sodium azide
Storage conditions short-term 4°C, long-term -20°C
Figure 1. Agonist-induced Threonine324/Serine327 phosphorylation of the Complement C5a... more

Figure 1. Agonist-induced Threonine324/Serine327 phosphorylation of the Complement C5a Receptor 1. Upper panel, HEK293 cells stably expressing the Complement C5a Receptor 1 (C5a1) were either not exposed or exposed to 1 µM specific Complement C5a receptor agonist CO28 or 10 μM Forskolin or 0.1 μM PMA (Phorbol 12-Myristate 13-Acetate) for 30 minutes. Cells were lysed and immunoblotted with the anti-pT324/pS327-C5a1 antibody (7TM0032A) at a dilution of 1:1000. Lower panel, blot was stripped and reprobed with the phosphorylation-independent anti-C5a1 antibody (7TM0032N-WB) at a dilution of 1:1000 to confirm equal loading of the gel.

Figure 2. Analysis of dose-dependent Complement C5a Receptor 1 phosphorylation using two phosphosite-specific antibodies. Upper two panels, HEK293 cells stably expressing the Complement C5a Receptor 1 (C5a1) were either not exposed or exposed to increasing concentrations of complement fragment C5a ranging from 1 nM to 100 nM for 30 minutes. Cells were lysed and immunoblotted with the anti-pT324/pS327-C5a1 antibody (7TM0032A) or anti-pS332/pS334-C5a1 antibody (7TM0032B) at a dilution of 1:1000. Lower panel, blot was stripped and reprobed with the phosphorylation-independent anti-C5a1 antibody (7TM0032N-WB) at a dilution of 1:1000 to confirm equal loading of the gel.

Figure 3. Analysis of agonist-dependent Complement C5a Receptor 1 phosphorylation using two phosphosite-specific antibodies. Upper two panels, HEK293 cells stably expressing the Complement C5a receptor 1 (C5a1) were either not exposed or exposed to 10 µM CO28 or 100 nM complement fragment C5a or 100 nM des-Arg C5a (C5a lacking the c-terminal arginine) for 30 minutes. Cells were lysed and immunoblotted with the anti-pT324/pS327-C5a1 antibody (7TM0032A) or anti-pS332/pS334-C5a1 antibody (7TM0032B) at a dilution of 1:1000. Lower panel, blot was stripped and reprobed with the phosphorylation-independent anti-C5a1 antibody (7TM0032N-WB) at a dilution of 1:1000 to confirm equal loading of the gel.

Figure 4. Immunocytochemical identification of Threonine324/Serine327 phosphorylation of the Complement C5a Receptor 1 in HEK293 cells. HEK293 cells stably expressing the Complement C5a Receptor 1 (C5a1) were either not exposed or exposed to 100 nM complement C5a and immunocytochemically stained with the anti-pT324/pS327-C5a1 antibody (7TM0032A) at a dilution of 1:200. Note, Threonine324/Serine327-phosphorylated C5a1 receptors were not detectable in untreated cells (0 min). Threonine324/Serine327-phosphorylated C5a1 receptors were seen as perinuclear clusters of vesicles after 30 min.

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