Abstract
Humoral immune responses in animals are often tightly controlled by regulated proteolysis. This proteolysis is exerted by extracellular protease cascades, whose activation culminates in the proteolytic cleavage of key immune proteins and enzymes. A model for such immune system regulation is the melanization reaction in insects, where the activation of prophenoxidase (proPO) leads to the rapid formation of eumelanin on the surface of foreign entities such as parasites, bacteria and fungi. ProPO activation is tightly regulated by a network of so-called clip domain serine proteases, their proteolytically inactive homologs, and their serpin inhibitors. In Anopheles gambiae, the major malaria vector in sub-Saharan Africa, manipulation of this protease network affects resistance to a wide range of microorganisms, as well as host survival. However, thus far, our understanding of the molecular make-up and regulation of the protease network in mosquitoes is limited. Here, we report the function of the clip domain serine protease CLIPB10 in this network, using a combination of genetic and biochemical assays. CLIPB10 knockdown partially reversed melanotic tumor formation induced by Serpin 2 silencing in the absence of infection. CLIPB10 was also partially required for the melanization of ookinete stages of the rodent malaria parasite Plasmodium berghei in a refractory mosquito genetic background. Recombinant serpin 2 protein, a key inhibitor of the proPO activation cascade in An. gambiae, formed a SDS-stable protein complex with activated recombinant CLIPB10, and efficiently inhibited CLIPB10 activity in vitro at a stoichiometry of 1.89:1. Recombinant activated CLIPB10 increased PO activity in Manduca sexta hemolymph ex vivo, and directly activated purified M. sexta proPO in vitro. Taken together, these data identify CLIPB10 as the second protease with prophenoloxidase-activating function in An. gambiae, in addition to the previously described CLIPB9, suggesting functional redundancy in the protease network that controls melanization. In addition, our data suggest that tissue melanization and humoral melanization of parasites are at least partially mediated by the same proteases.
Highlights
Melanization, the biochemical formation and deposition of melanin fulfills diverse biological functions in living organisms (Cerenius and Soderhall, 2004; Vavricka et al, 2010; Sugumaran and Barek, 2016; Pavan et al, 2020)
Quantification of melanotic areas per abdomen demonstrated a significant reduction in melanization in dsSRPN2/dsCLIPB10 as compared to dsSRPN2-treated mosquitoes (Figure 1B)
We focused our analysis on CLIPB10, based on the results of previous targeted reverse genetic screens and phylogenetic analyses of CLIPBs performed by us and others (Paskewitz et al, 2006; An et al, 2011; Cao et al, 2017)
Summary
Melanization, the biochemical formation and deposition of melanin fulfills diverse biological functions in living organisms (Cerenius and Soderhall, 2004; Vavricka et al, 2010; Sugumaran and Barek, 2016; Pavan et al, 2020). Subsequent genetic studies identified single genes whose knockdown (kd) triggers a potent melanotic response against Plasmodium ookinetes (Osta et al, 2004; Michel et al, 2005; Frolet et al, 2006; Nakhleh et al, 2017a), drawing considerable attention to the potential application of this response in controlling vector competence. The non-vector mosquito, Anopheles quadriannulatus, was shown to trigger a potent immune response to Plasmodium ookinetes characterized by a significant melanization of P. berghei ookinetes and occasionally of P. falciparum (Habtewold et al, 2008). The infection-induced melanization in An. gambiae is tightly regulated by the complement-like pathway, the thioester-containing protein 1 (TEP1), which upon activation is deposited on the surface of entities that are recognized as damaged or foreign (Blandin et al, 2004; Yassine et al, 2012a; Povelones et al, 2013). Melanin formation on surfaces of microbes is thought to hinder their intake of nutrients, while toxic intermediates, such as reactive oxygen and reactive nitrogen species, may cause cellular damage (Nappi et al, 2009)
Sign-in/Register to view highlights & summary 
Published Version (
Free)
Talk to us
Join us for a 30 min session where you can share your feedback and ask us any queries you have
Schedule a call