Abstract
In mammals, the bioactive fragment C3a, released from C3 during complement activation, is a potent mediator of inflammatory reactions and exerts its functional activity through the specific binding to cell surface G protein-coupled seven-transmembrane receptors. Recently, we demonstrated a Ciona intestinalis C3a (CiC3a)-mediated chemotaxis of hemocytes in the deuterostome invertebrate Ciona intestinalis and suggested an important role for this molecule in inflammatory processes. In the present work, we have cloned and characterized the receptor molecule involved in the CiC3a-mediated chemotaxis and studied its expression profile. The sequence, encoding a 95,394 Da seven-transmembrane domain protein, shows the highest sequence homology with mammalian C3aRs. Northern blot analysis revealed that the CiC3aR is expressed abundantly in the heart and neural complex and to a lesser extent in the ovaries, hemocytes, and larvae. Three polyclonal Abs raised in rabbits against peptides corresponding to CiC3aR regions of the first and second extracellular loop and of the third intracellular loop react specifically in Western blotting with a single band of 98-102 kDa in hemocyte protein extracts. Immunostaining performed on circulating hemocytes with the three specific Abs revealed that CiC3aR is constitutively expressed only in hyaline and granular amoebocytes. In chemotaxis experiments, the Abs against the first and second extracellular loop inhibited directional migration of hemocytes toward the synthetic peptide reproducing the CiC3a C-terminal sequence, thus providing the compelling evidence that C. intestinalis expresses a functional C3aR homologous to the mammalian receptor. These findings further elucidate the evolutionary origin of the vertebrate complement-mediated proinflammatory process.
Highlights
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A basic local alignment search tool analysis of this sequence in the Ciona genome, version 1.0, revealed that the CiC3aR regions between the nt 1–750 and 1673–3053 were present in scaffolds 455 and 438, respectively, whereas the region between nt 751-1672 was not found in any scaffold
A further analysis conducted in the National Center for Biotechnology Information database revealed the presence of a 1536-bp C. intestinalis cDNA clone [34] corresponding to the 1534 –3071 region of the presumptive CiC3aR
Summary
EL, extracellular loop; CiC3a, C. intestinalis C3a; JTT, Jones-Taylor-Thornton; IL, intracellular loop. C3-like genes have been identified in different species of invertebrates [21], and in limited instances, C3-mediated functions have been reported in these organisms [22,23,24,25]. Three polyclonal Abs raised against peptides reproducing different portions of the deduced amino acid sequence of this receptor have been used in chemotaxis experiments, Western blot analysis, and immunostaining of circulating hemocytes. The results of these experiments demonstrate for the first time the presence and the functional activity of a C3aR in an invertebrate species
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