Abstract
The complement-like protein thioester-containing protein 1 (TEP1) is a key factor in the immune response of the malaria vector Anopheles gambiae to pathogens. Multiple allelic variants of TEP1 have been identified in laboratory strains and in the field, and are correlated with distinct immunophenotypes. TEP1 is tightly regulated by conformational changes induced by cleavage in a protease-sensitive region. Cleaved TEP1 forms exhibit significant variation in stability from hours to days at room temperature. In particular, the refractory allele TEP1*R1 is significantly more stable than the susceptible allele TEP1*S1. This raises the question of whether the stability of cleaved TEP1 is linked to allelic variation and varying immunophenotypes. We have analyzed the stability of the cleaved form of additional TEP1 alleles and constructs. We show that stability is correlated with allelic variation within two specific loops in direct proximity to the thioester bond. The variable loops are part of an interface between the TED and MG8 domains of TEP1 that protect the thioester from hydrolysis. Engineering specific disulfide bonds to prevent separation of the TED-MG8 interface stabilizes the cleaved form of TEP1 for months at room temperature. Cleaved TEP1 forms a soluble complex with a heterodimer of two leucine-rich repeat proteins, LRIM1 and APL1C, and precipitates in the absence of this complex. The molecular structure and oligomeric state of the TEP1/LRIM1/APL1C complex is unclear. The C-terminal coiled-coil domain of the LRIM1/APL1C complex is sufficient to stabilize the cleaved form of TEP1 in solution but cleaved forms of disulfide-stabilized TEP1 do not interact with LRIM1/APL1C. This implies that formation of the TEP1cut/LRIM1/APL1C complex is related to the conformational change that induces the precipitation of cleaved TEP1.
Highlights
The mosquito Anopheles gambiae is the principal malaria vector in Sub-Saharan Africa
We show that engineered disulfides within the thioester domain (TED)-CUB-MG8 superdomain can stabilize TEP1cut similar to LRIM1/APL1C. These results suggest that the formation of the TEP1cut/LRIM1/ APL1C complex requires a conformational change involving dissociation of the TED-MG8 interface that is directly related to the conformational change leading to thioester hydrolysis and precipitation of TEP1cut in the absence of LRIM1/APL1C
We previously showed that a chimeric protein replacing the TED of thioester-containing protein 1 (TEP1) R1 with TEP1 S1 had the same stability as TEP1 S1 [8], but this does not determine which of the three loops are responsible for this variable stability
Summary
The mosquito Anopheles gambiae is the principal malaria vector in Sub-Saharan Africa. The immune response of A. gambiae is a significant factor influencing the vectoral capacity of mosquitoes to malaria parasites (genus Plasmodium). Plasmodium ookinetes invade and traverse the midgut epithelium, whereupon they face a robust complement-like immune response [1]. The complement-like factor thioester-containing protein 1 (TEP1) binds to the surface of Plasmodium ookinetes. The reactive thioester bond, a feature of the TEP protein family including α2macroglobulins and complement factors, is protected from hydrolysis in the full-length protein by an interface formed between the TED and the MG8 domain [2]. A triangular arrangement of the TED, CUB and MG8 domains forms a ‘superdomain’ that is conserved between TEP1 and mammalian complement factor C3 [3, 4]
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