Malaria parasite LIMP protein regulates sporozoite gliding motility and infectivity in mosquito and mammalian hosts
Abstract
Gliding motility allows malaria parasites to migrate and invade tissues and cells in different hosts. It requires parasite surface proteins to provide attachment to host cells and extracellular matrices. Here, we identify the Plasmodium protein LIMP (the name refers to a gliding phenotype in the sporozoite arising from epitope tagging of the endogenous protein) as a key regulator for adhesion during gliding motility in the rodent malaria model P. berghei. Transcribed in gametocytes, LIMP is translated in the ookinete from maternal mRNA, and later in the sporozoite. The absence of LIMP reduces initial mosquito infection by 50%, impedes salivary gland invasion 10-fold, and causes a complete absence of liver invasion as mutants fail to attach to host cells. GFP tagging of LIMP caused a limping defect during movement with reduced speed and transient curvature changes of the parasite. LIMP is an essential motility and invasion factor necessary for malaria transmission.
https://doi.org/10.7554/eLife.24109.001Introduction
Malaria parasites rely on gliding motility for migration through and invasion of diverse cells in two different host species: mosquitoes and humans. Ookinetes and sporozoites, the motile forms of the malaria parasite, are morphologically distinct but share core components of a gliding motility apparatus. The glideosome, an actin-myosin motor anchored within the inner membrane complex (IMC), is connected to the substrate via adhesins localised at the parasite surface (Bargieri et al., 2014; Baum et al., 2008; Harding and Meissner, 2014; Kono et al., 2013, 2012). As shown in the related pathogen Toxoplasma gondii, adhesins are discharged upon contact with host cells from specialised secretory organelles, the micronemes (Carruthers and Sibley, 1997). Some malaria micronemal proteins, like the ookinete SOAP (Dessens et al., 2003) and WARP proteins (Yuda et al., 2001; Li et al., 2004), are secreted into the extracellular milieu, while others—CTRP for example (Yuda et al., 1999; Dessens et al., 1999)—are retained in the plasma membrane via transmembrane domains, from where they can engage host cell receptors. Translocated backwards along the cell surface during gliding, TM domain-containing proteins are continuously shed by rhomboid and subtilisin-like serine proteases (Baum et al., 2008; Brossier et al., 2005; Baker et al., 2006; Ejigiri et al., 2012) and deposited onto the substrate as gliding trails that can be detected by electron microscopy (Stewart and Vanderberg, 1992) or immunofluorescence (Ejigiri et al., 2012; Kappe et al., 1999; Kariu et al., 2006). Many factors involved in adhesion, motility and invasion of ookinetes and sporozoites are largely expressed in a life-cycle-dependent manner: they include CTRP (Yuda et al., 1999; Dessens et al., 1999), WARP (Yuda et al., 2001; Li et al., 2004; Ecker et al., 2008), SOAP (Dessens et al., 2003), CHT1 (Li et al., 2004; Dessens et al., 2001) and MAOP (Kadota et al., 2004) in the ookinete; in the sporozoite AMA1 (Giovannini et al., 2011; Bargieri et al., 2013; Silvie et al., 2004), TRAP (Kappe et al., 1999; Sultan et al., 1997; Matuschewski et al., 2002), MAEBL (Kariu et al., 2002; Saenz et al., 2008), SPECT (Ishino et al., 2004), SPECT2 (Ishino et al., 2005a), GEST (Talman et al., 2011) and P52 (Ishino et al., 2005b; Annoura et al., 2014; Labaied et al., 2007a; van Dijk et al., 2005); CelTOS is common to both (Jimah et al., 2016). Additional surface proteins implicated in parasite motility and host cell invasion include S6/TREP/UOS3 (Mikolajczak et al., 2008; Steinbuechel and Matuschewski, 2009; Combe et al., 2009), TLP (Hellmann et al., 2011; Moreira et al., 2008; Heiss et al., 2008; Lacroix and Ménard, 2008), PCRMP1 and 2 (Thompson et al., 2007), the rhoptry-resident proteins TRSP (Kaiser et al., 2004; Labaied et al., 2007b) and RON4 (Giovannini et al., 2011), the GPI-anchored circumsporozoite protein (CSP) of the sporozoite and the small solute transporter PAT (Kehrer et al., 2016a) (Supplementary file 1). If, and how these different factors interact with each other, and in turn with host cell receptors to coordinate efficient gliding motility and host cell invasion is poorly understood (Meissner et al., 2013). Recombinant protein and peptide competition studies have revealed binding of CSP to mosquito salivary glands (Myung et al., 2004; Sidjanski et al., 1997) through mosquito heparan sulphate (Sinnis et al., 2007) and a TRAP-saglin interaction to allow efficient invasion of this organ (Ghosh et al., 2009). In the liver, heparan sulphate proteoglycans (HSPGs) on the surface of different cells but also on the extracellular matrix have been proposed to act as main receptors for sporozoites. Again, CSP and TRAP are key players in sporozoite sequestration by interacting with the cell’s HSPGs (Prudêncio et al., 2006; Morahan et al., 2009; Frevert et al., 1993; Coppi et al., 2007), but also with fetuin-A on hepatocyte membranes in the case of TRAP (Jethwaney et al., 2005).
Gliding motility and cell invasion mechanisms are conserved among apicomplexan parasites. While intracellular motor, IMC and pellicle components are shared between Toxoplasma gondii and Plasmodium parasites (Harding and Meissner, 2014), many of the Plasmodium adhesins (14 out of 24) lack clearly recognisable homologs in T. gondii (Supplementary file 1). Here, we identify the 110 amino acid LIMP protein as a crucial surface protein for gliding motility in the rodent malaria model P. berghei. LIMP (the name refers to a peculiar gliding phenotype in the sporozoite arising from epitope tagging of the endogenous protein) is a key factor for sporozoite infectivity in the mosquito and the rodent host: LIMP regulates gliding motility and salivary gland invasion; it enables sporozoites to adhere to, traverse and invade host hepatocytes. Conserved in human malaria parasites and related apicomplexans, the protein could be a target for transmission-blocking vaccines in a manner developed for CelTOS (Espinosa et al., 2017) or TRAP (Rampling et al., 2016).
Results
limp is maternally supplied to developing ookinetes
In recent genome-wide studies, we have identified more than 100 mRNAs encoding known and putative surface proteins to be under translational control during transmission of P. berghei gametocytes from the rodent to the mosquito host (Mair et al., 2006, 2010; Guerreiro et al., 2014). One of these transcripts encodes the protein PBANKA_0605800 (from here on forward referred to as LIMP). LIMP is encoded by an 1194 basepair long gene in the P. berghei ANKA strain. The gene (Figure 1A) comprises six exons and five introns (this organisation is conserved throughout the genus) and encodes a protein of 110 amino acids (aa) with a 22 aa long signal peptide (Figure 1B) and a molecular weight of 13 kDa. Ab initio protein structure predictions (Combet et al., 2000; Xu and Zhang, 2012) indicate that LIMP (I23 to G110) consists of three beta sheets opposed to two α-helices (Figure 1C). LIMP is highly conserved among the various Plasmodium species (Figure 1B; www.plasmodb.org) (Aurrecoechea et al., 2009); similarly short proteins are present in related apicomplexan parasites, where the homology is focused on a 22 amino acid proline-rich region adjacent to the signal peptide (Figure 1—figure supplement 1).
limp was found downregulated in a gene knock-out for the translational repressor DOZI and its mRNA enriched in an RNA-immunoprecipitation (RIP) of CITH (Mair et al., 2006, 2010; Guerreiro et al., 2014), suggesting that limp mRNA is kept translationally repressed in female gametocytes until activated during ookinete development, or later. To assess experimentally when limp is translated, we tagged the endogenous gene at the C terminus with GFP, thus leaving the fusion under the transcriptional control of the native promoter in this haploid protozoan (Figure 1—figure supplement 2); then, we followed its expression. In this mutant, limp::gfp is the only source for LIMP (Figure 1D and Figure 1—figure supplement 2). We found no protein expression in asexual stage parasites or gametocytes; limp::gfp is translated in the ookinete stage and its expression is visible in crystalloids (transient and putative storage organelles of the ookinete) (Dessens et al., 2011) and the surface; the protein produced a faint ‘dusting’ on the surface of midgut and salivary gland sporozoites (Figure 1E; see also Figure 4). In agreement with previously published results (Otto et al., 2014), limp mRNA was not detected in asexual blood stages; mRNA is however present in gametocytes (while protein is not) and in ookinetes (where protein is present) (Figure 1F); this is consistent with limp being translationally repressed and maternally provided to the developing ookinete. Western blot analysis of ookinete material confirmed expression of a GFP fusion protein of the expected size (Figure 1G). Parasites expressing LIMP::GFP showed no defects in liver stage development in vitro nor during transmission to the rodent host by mosquito bite (Figure 1—figure supplement 3).
limp gene deletion mutants suffer cumulative population loss during mosquito and rodent passage
In order to appreciate the function of LIMP for mosquito stage development and/or invasion of the Anopheles vector, we generated two independent gene knock-out (KO) mutant lines—Δlimp-a (Δa) and Δlimp-b (Δb)—replacing the entire open reading frame (ORF) with a pyrimethamine resistance cassette in the reference parasite line Fluo-frmg (the Fluo-frmg clone produces GFP+ male and RFP+ female gametocytes) (Mair et al., 2010) (Figure 2—figure supplement 1). The absence of LIMP did not affect asexual blood-stage development, gametocyte numbers nor female to male ratios (Figure 2—figure supplement 2), and the capacity of Δlimp parasites to produce ookinetes was comparable to that of wildtype (WT) lines; in vitro zygote to ookinete conversion rates ranged from 55% to 91% (Figure 2A). However, following a mosquito blood meal, infection rates (oocyst numbers per mosquito) were reduced below 50% (Figure 2B), while the number of oocyst-derived midgut sporozoites per oocyst remained unchanged (Figure 2C); ookinete development and oocyst sporulation therefore do not require LIMP. Δlimp sporozoites did not significantly accumulate in the haemolymph (Figure 2D), but showed a 10-fold reduction in salivary gland invasion (Figure 2E). Our results demonstrate a role for LIMP during mosquito midgut colonisation by the ookinete, and a crucial function for the protein during salivary gland invasion, but not for development; neither ookinete nor sporozoite formation were affected by the absence of LIMP. We next tested whether the salivary gland invasion defect extended to invasion of the mammalian host. To this end, naive mice were infected by intravenous (i.v.) injection of 3,500 hand-dissected sporozoites (Figure 2F). WT-infected mice established normal blood-stage parasitaemias, while KO-infected mice never did. Mice injected i.v. with Δlimp salivary gland sporozoites showed no parasite load in the liver at 44 hr post-infection (p.i.) when determined by qPCR of the P. berghei ANKA 18S gene (Figure 2G), corroborating the notion that mutants had failed to invade the liver. In vitro hepatocyte infection assays supported the in vivo data; Δlimp salivary gland sporozoites did not establish exoerythrocytic forms (EEFs) inside Huh7 hepatoma cells (Figure 2H).
Δlimp sporozoites are impaired in hepatocyte transmigration, adhesion and invasion and do not glide
Our parasite transmission data clearly established a role for LIMP during the traversal of host barriers, but no role in developmental progression. Mosquito midgut colonisation was strongly affected with a 50% reduction in oocyst numbers, and infections of the mosquito’s salivary glands and the rodent host’s liver were almost abolished in the absence of LIMP. Therefore, the protein’s role lies likely in motility. Especially, the near-absence of salivary gland sporozoites in Δlimp mutants suggested that LIMP is a novel and key gliding motility factor in the sporozoite. Plasmodium and related apicomplexan parasites move by gliding motility, which requires the establishment and dissolution of parasite-host cell contact points and the ordered turn-over of such adhesion sites (Münter et al., 2009); in the case of TRAP, this is mediated by rhomboid protease cleavage within the transmembrane domain severing the connection between parasite and host (Ejigiri et al., 2012). We therefore examined the parasite’s motility behaviour in different assays: the sporozoite’s ability to traverse, invade and adhere to host hepatocytes; the quantification of CSP trails as a measure of sporozoite gliding ability; and determination of sporozoite movement patterns and speed by live microscopy.
limp KO sporozoites showed a complete failure to traverse hepatocytes when determined by FACS analysis; the percentage of Dextran+ host cells (the polysaccharide enters through cell membrane injury sites caused by invading sporozoites) was not different from levels obtained from cells incubated with non-infected mosquito salivary gland material (Figure 3A). Mutant sporozoites also showed a clear defect in adherence to Huh7 cells (Figure 3B) together with greatly reduced hepatocyte invasion (Figure 3C), explaining the failure to establish an infection in the rodent host. Next, we performed a gliding motility assay that is based on the detection of trails of the surface protein CSP, which is deposited onto microscope coverslips by moving sporozoites. KO parasites were severely impaired in gliding motility, evident by the large number of completely immotile parasites as well as the number of gliding trails of the few moving ones (Figure 3D–E).
Morphologically, KO parasites are normal. Transmission electron microscopy (TEM) studies of Δlimp sporozoites revealed no ultrastructural defects in key components of the gliding motility machinery. The arrangement of the plasma membrane (PM), inner membrane complex (IMC), subpellicular microtubules as well as secretory vesicles (micronemes and rhoptries) was unchanged (Figure 3F). As expected, Δlimp sporozoites were found within the mosquito’s salivary gland parenchyma, confirming that some mutants can invade the salivary glands and are not merely attached to the outer surface of the glands facing the haemocoel (Figure 3G).
LIMP::GFP localises to the sporozoite surface and supports wild-type life cycle progression
GFP-tagging of the endogenous gene exposed both intracellular and surface localisation (Figure 1E). In the ookinete LIMP::GFP highlighted, apart from faint surface staining, foci that correspond to crystalloids, transient ookinete stage-specific organelles that provide protein and lipid material for sporozoite formation in the oocyst (Guerreiro et al., 2014; Dessens et al., 2011; Lavazec et al., 2009; Santos et al., 2016; Saeed et al., 2015; Lin et al., 2013; Saeed et al., 2013). When we performed IFAs on limp::gfp sporozoites recovered from salivary glands, fluorescence was found in a dusted, speckled distribution along the entire length of the parasite (Figure 1E and Figure 4A). LIMP::GFP was detectable both with and without Triton X-100 permeabilisation (Figure 4A), a clear indication for parasite cell surface positioning of LIMP in a manner resembling TRAP (which is secreted from micronemes) and CSP (Figure 4—figure supplement 1) (Ejigiri et al., 2012). We confirmed this observation with two additional mutant lines, varying position and size of the tags: mcherry::limp (Figure 4—figure supplement 2) and limp::myc (Figure 4—figure supplement 3). Both showed a normal range of oocysts as well as midgut and salivary gland sporozoite numbers (Figure 4—figure supplement 1). The staining patterns of tagged LIMP in all three transgenic lines was identical (Figure 4A), showing that trafficking of tagged LIMP does not alter with tag size nor position (N- versus C-terminus), and all supporting—opposed to the knock-out—infection of the mosquito host. Using an immuno-electron microscopy (immuno-EM) approach (Figure 4B), we corroborated LIMP::GFP localisation in three independent staining experiments with three different parasite samples. Seventy-six percent of gold particles (from a total of 281) were associated with the parasite PM, 11% outside of parasites; 13% were intracellular although not clearly associated with any specific organelle.
Given the surface localisation of LIMP, the severe attachment and gliding defects of Δlimp parasites (Figure 3B,D–E), we wanted to examine the role of LIMP in live motility assays. Owing to the scarcity of Δlimp salivary gland sporozoites, we performed live in vitro gliding assays using haemolymph sporozoites instead, as these were more readily available, and compared them to WT and limp::gfp haemolymph sporozoites. Again, exceptionally few gene deletion sporozoites showed normal circular movement while the vast majority were found floating in the medium (Figure 4C), unable to attach to the glass bottom of a 96-well plate.
As expected, the limp::gfp haemolymph sporozoite population displayed a normal distribution of gliding motility patterns (Figure 4C). But when we analysed the speed of productively moving WT and limp::gfp sporozoites we found, surprisingly, limp::gfp sporozoites to move significantly slower (Figure 4D) despite limp::gfp salivary gland sporozoites producing normal numbers of CSP trails (Figure 4E–F). The presence of high concentrations of anti-GFP antibodies (potentially targeting LIMP::GFP) nor control IgGs affected CSP shedding (Figure 4E) or in vitro hepatocyte invasion by limp::gfp sporozoites (Figure 4G), mimicking a published TRAP study showing no effect of anti-TRAP antibodies on gliding motility (Gantt et al., 2000), while anti-CSP antibodies stopped sporozoite motility in vitro and blocked hepatocyte invasion in vivo (Stewart et al., 1986). Finally, we explored the possibility that LIMP::GFP is shed from the parasite surface during gliding in a manner resembling CSP or TRAP. To this end, we coated microscope slides with anti-GFP antibodies used for sporozoite immunofluorescence. No gliding trails were detected in this assay, suggesting that GFP-tagged LIMP is not shed from the parasite surface, or perhaps is shed at levels below the detection limit of this assay.
LIMP::GFP parasites glide with a ‘limp’
While the CSP trail-based motility analyses failed to flag the motility defect of limp::gfp parasites, live motility assays of salivary gland sporozoites revealed a peculiar feature in this strain: the number of moving and partially moving parasites was similar to WT (Figure 5A), but the speed was reduced by more than 35% when quantified by live microscopy (Figure 5B). Upon closer examination of trajectories of gliding paths, we identified a higher number of limp::gfp parasites with irregular trails and wider circumferences instead of tight, concentric rings typical for WT parasites (sporozoite tracks are visualised by connecting lines between two consecutively tracked positions) (Figure 5C). This means that WT sporozoites complete one full circle within a lower number of frames than the slower limp::gfp sporozoites. As a result, the circular tracks of WT sporozoites are tighter because the tracked positions are further apart than those of limp::gfp sporozoites. Typically, WT parasites move continuously in a circular fashion following their crescent shape (Video 1). limp::gfp sporozoites on the other hand produced a peculiar ‘limp’ (Video 2)—whence the gene and protein designation is derived. This limping motility is characterised by a failure of the sporozoite to detach with the rear end, while the front end continues moving forward thus leading to a transient loss of curvature and a straightening of the parasites, whereby the body size remains unchanged. limp::gfp sporozoites show an accentuated frequency of these cell stretching events (Figure 5D–E), which results in a temporary increase of sporozoite front-to-rear end distance when the parasite fails to detach (Figure 5F). While less than 22% of WT sporozoites exhibit one or more limps during 100 s of gliding, 62% of limp::gfp sporozoites limped at least three times during that period (Figure 5D). This effect was specific for C-terminally GFP-tagged LIMP, while both the smaller C-terminal MYC-tag or the N-terminal mCherry-tag supported WT movement and did not produce the staccato movement of limp::gfp (Figure 5D–E). Consequently, the average speed of mcherry::limp and limp::myc parasites was similar to WT and thus faster than that of limp::gfp sporozoites (Figure 5B).
C-terminal GFP tagging occludes crucial surface areas of LIMP
The sporozoite motility data showed that C-terminal GFP tagging of LIMP resulted in a reduced detachment efficiency. LIMP contains three N-terminal beta sheets and two anti-parallel helices (G60-K83 and K89-N109) at the C-terminus (Figure 1C and Figure 6—figure supplement 1). This structure is conserved among all Plasmodium LIMP members (Figure 1B) and may provide surface and interaction sites to other parasite proteins, or proteins of the hosts. In order to compare the stability of WT LIMP structure and the effect of the different tags, we performed molecular dynamics simulations over a time period of 100 ns. The WT protein maintained a stable fold, while LIMP::GFP showed a clear destabilisation of helix 1 (G60-K83) resulting in a kink and a subsequent break of the helix between H71 and Y75 (Figure 6—figure supplement 1). This is exemplified by the increased distance between the C-α atoms of these two amino acids (Figure 6—figure supplement 1). Furthermore, the stable intra-helical H-bonds were lost in helix 1 (G60-K64, I72-E76 and E73-T77) and helix 2 (S95-K99) of LIMP::GFP (Figure 6—figure supplement 1). In addition, the GFP tag occludes the surface area of LIMP helices, while neither MYC nor mCherry tags interfere with this surface (Figure 6 and Figure 6—figure supplement 2). The loss of structural integrity and solvent accessibility in the GFP fusion protein is likely the cause for the reduced efficiency in detachment and limping motility.
Discussion
Here, we have identified a novel Plasmodium protein, LIMP, with a core function for gliding motility and infection in the rodent P. berghei malaria parasite model. While genes encoding proteins involved in invasion and gliding motility are assumed to be transcribed and translated when needed, recent studies highlighted many mRNAs encoding motility and invasion proteins to be transcribed and translationally repressed in the female gametocyte, and thus maternally provided to the developing ookinete and oocyst (Ecker et al., 2008; Guerreiro et al., 2014; Santos et al., 2016; Saeed et al., 2013; Rao et al., 2016; Sebastian et al., 2012; Raine et al., 2007). LIMP is one of these factors. Ookinetes that lack LIMP displayed a 50% reduction in parasite burden in mosquito midguts. The resulting haemolymph sporozoites were heavily affected in their motility and ability to invade and parasitise the mosquito salivary glands; the small population of salivary gland sporozoites was incapable of establishing a productive infection in hepatocytes, neither in vitro nor in vivo. In sporozoites, LIMP localises to the parasite plasma membrane, as determined by examination of three different tagged parasite lines (limp::gfp, mcherry::limp and limp::myc) and immuno-gold EM studies. The protein is probably of low abundance, and LIMP is yet to be discovered in the sporozoite proteomes from the rodent parasite species P. berghei and P. yoelii or the human parasite P. falciparum (Swearingen et al., 2016; Hall et al., 2005; Lasonder et al., 2008; Lindner et al., 2013).
We propose that LIMP could be involved in the attachment of sporozoites to the substrate, and perhaps regulate efficient turnover of attachment sites in gliding parasites. The underlying requirement for gliding, cell traversal and invasion of malaria parasites is adhesion to the substrate, either artificial ones such as glass or plastic, or cells from various host tissues (midgut and salivary gland epithelia of the mosquito; mammalian skin, liver sinusoidal cells or hepatocytes) (Singer and Frischknecht, 2012; Vaughan et al., 2008). In Plasmodium sporozoites—the key model for understanding gliding motility—adhesion is a three-step process: initial attachment at the apical (front) or posterior (rear) end followed by a secondary adhesion site at the opposite end; the apical end then moves slightly forward and the sporozoite flips over on one of its sides, thus increasing the area of contact between the sporozoite body and the substrate; finally, a tertiary attachment point is made at the centre of the parasite. The primary step of adhesion is dependent on intracellular actin dynamics, as the induction of actin polymerisation leads to weaker adhesion (Hellmann et al., 2013; Hegge et al., 2012, 2010), and requires cell surface proteins such as TRAP and S6/TREP/UOS3; they are important for initial in vitro adhesion and this function is associated with the interaction of the proteins’ von-Willebrand-factor-A extracellular adhesive domains with the substrate (Hegge et al., 2010). TRAP-deficient parasites adhere preferentially with their front end, while sporozoites lacking S6/TREP/UOS3 show no preference for apical or rear end initial adhesion. Moreover, their differential spatial interaction with actin filaments suggests these proteins cannot compensate for one another during adhesion and motility (Hegge et al., 2012). Another protein, TLP, solely stabilises newly formed adhesion sites and/or increases the speed of adhesion formation, thereby augmenting continued adhesion formation during gliding (Hegge et al., 2010). HSP20 has been implicated in the regulation of the dynamics of parasite adhesion site formation and rupture. Parasites lacking HSP20 show longer adhesion sites and slower gliding motility, while in vitro cell traversal and invasion is unaffected (Montagna et al., 2012). Δlimp parasites adhere less to hepatoma cells or glass surfaces implying that LIMP is required for the establishment of initial adhesion contacts with the substrate, thereby affecting the subsequent events of motility and invasion; in that sense, it has an equivalent function to TRAP (Münter et al., 2009).
After attachment to the substrate, continuous parasite motility requires the continuous turnover of adhesion sites. Strong adhesion forces at the rear end of the sporozoite during gliding can lead to temporal arrest, causing stretching of the parasite when it pulls forward (Münter et al., 2009). Unlike Δtrap mutants, the limp::gfp mutant is able to glide, albeit with reduced speed caused by frequent stretching events as a result of a de-adhesion defect at its rear end. Fusing GFP to LIMP allowed us to uncover, serendipitously, this additional function for the protein. However, the fact that limp::gfp parasites complete the life cycle (no differences exist in parasite numbers in mosquitoes or in prepatent period after mosquito bite) suggests that LIMP::GFP still exerts its essential role in sporozoite biology. One can therefore also be confident that its localisation at the sporozoite PM reflects the true site of action of untagged LIMP protein. Tagging of LIMP with two alternative tags of different sizes fused to either the N- or C-terminus (mCherry and MYC, respectively) replicated the subcellular localisation of LIMP::GFP, and shows that the limping phenotype is specifically induced by the large GFP tag positioned at the C-terminus of the protein; both mCherry and MYC-tagged lines behaved as WT parasites in every way analysed. We have attempted to generate anti-LIMP antibodies in rabbits to further corroborate LIMP localisation but the resulting sera failed to reveal antigen-specific, reliable staining.
The phenotype of limp::gfp parasites highlights the importance of LIMP for coordinated and timely detachment of the sporozoite from its substrate, thereby allowing uninterrupted, smooth gliding. Perhaps, LIMP is a regulator of TRAP, or acts in concert with TRAP and related family members. Alternatively, LIMP could be acting entirely independently. Both scenarios highlight how little we understand about formation of adhesion sites, their turnover and the generation of force within the parasite, or how different surface proteins co-operate. LIMP is essential for parasite transmission by facilitating productive gliding motility required for the traversal of mosquito and mammalian tissues, as well as invasion of the mosquito salivary glands and liver cells in the vertebrate host (Figure 7). Several secreted proteins of parasite origin play a role in one or more of these processes: CTRP (Yuda et al., 1999; Dessens et al., 1999; Templeton et al., 2000), MAOP (Kadota et al., 2004) and SOAP (Dessens et al., 2003) in the ookinete; MAEBL (Kariu et al., 2002; Saenz et al., 2008), SPECT (Ishino et al., 2004), SPECT2 (Ishino et al., 2005a), P52 (Ishino et al., 2005b; Labaied et al., 2007a) and TRAP (Ejigiri et al., 2012; Kappe et al., 1999; Sultan et al., 1997; Matuschewski et al., 2002; Mota et al., 2001) in the sporozoite; and CelTOS (Kariu et al., 2006) in both the ookinete and the sporozoite (Supplementary file 1). Finding LIMP binding partners will constitute an important first step to unravelling its precise molecular mechanism of action and will rely on co-immunoprecipitation or proximity-dependent biotinylation approaches (Kehrer et al., 2016b). LIMP is conserved across different malaria parasite species, and proteins with lower homology are present in apicomplexan parasites of humans (T. gondii) and livestock (Neospora or Eimeria). The protein is thus an obvious target for intervention strategies that impede the gliding motility machinery.
Materials and methods
Experimental
Request a detailed protocolIn Instituto de Medicina Molecular (iMM, Lisbon, Portugal), animal experimentation protocols were approved by the iMM Animal Ethics Committee (under authorisation AEC_2010_018_GM_Rdt_General_IMM) and the Portuguese authorities (Direção Geral de Alimentação e Veterinária). Animal experiments performed in Leiden University Medical Center (LUMC, Leiden, The Netherlands) were approved by the Animal Experiments Committee of the Leiden University Medical Center (DEC 10099; 12042; 12120). At the University of Heidelberg Medical School (Heidelberg, Germany) animal work was approved by the German authorities (Regierungspräsidium Karlsruhe; 35–9185.81/G-266/16) and performed in compliance with FELASA guidelines and regulations. All animal work was in accordance with EU regulation. Animals used were female Balb/c (RRID:IMSR_CRL:28), OF-1 (RRID:IMSR_CRL:612) and NMRI (RRID:IMSR_CRL:605) mice (6–8 weeks old) bred at Charles River or Janvier Labs, France.
Reference P. berghei ANKA lines
Request a detailed protocolFour P. berghei ANKA parasite lines were used (for details see RMgm database at www.pberghei.eu): line HPE, a non-gametocyte producer clone (Janse et al., 1989); line 820cl1m1cl1 (Fluo-frmg; RMgm-164) (Mair et al., 2010) expressing RFP under the control of a female gametocyte-specific promoter and GFP under the control of a male gametocyte-specific promoter; line 259cl1 (PbGFPcon; RMgm-5) (Franke-Fayard et al., 2004) expressing GFP under the control of the constitutive eef1a promoter; and line cl15cy1, which is the reference parent line of P. berghei ANKA (Janse et al., 2006a).
Cell lines
Request a detailed protocolHuh7 cells (RRID:CVCL_0336) were obtained from the Japanese Collection of Research Bioresources Cell Bank (JCRB Cell Bank), from the National Intitutes of Biomedical Innovation, Health and Nutrition (NIBIOHN). General information about these cells can be found here: http://cellbank.nibiohn.go.jp/~cellbank/en/search_res_det.cgi?ID=385#. Huh7 is an immortal cell line derived from a well-differentiated human hepatocellular carcinoma. It has an epithelial-like morphology and was originally isolated from a liver hepatoma tissue in a 57-year-old Japanese male in 1982. The line was established by Nakabayashi and collaborators (Nakabayashi et al., 1982). Cell authenticity was confirmed by the Wellcome Trust Sanger Institute under the Catalogue Of Somatic Mutations In Cancer (COSMIC) Cell Lines Project. Identity data, including STR profiling, is available at: http://cancer.sanger.ac.uk/cell_lines/sample/overview?id=907071#overview.
This cell line is not listed in the International Cell Line Authentication Committee (ICLAC) Database of Cross-Contaminated or Misidentified Cell Lines. It was regularly checked throughout the duration of this study for mycoplasma contamination using the VenorGeM OneStep – Mycoplasma Detection Kit for conventional PCR (Minerva Biolabs GmbH, #11-8025) and no evidence of contamination was ever found.
Reverse transcriptase-PCR (RT-PCR)
Request a detailed protocolTo investigate the transcription pattern of limp by RT-PCR, RNA from different life cycle stages were obtained using TRIzol Reagent (Ambion, #15596). Reverse transcription was primed with random primers and oligo-d(T) using SuperScript II Reverse Transcriptase (Invitrogen, #18064). Oligonucleotide primers used in life cycle RT-PCRs are shown in Supplementary file 2A.
Generation of limp gene deletion mutants
Request a detailed protocolDeletion of limp (PBANKA_0605800) was performed with a standard replacement construct (Janse et al., 2006b) using a modified plasmid pL0001 (www.mr4.com), which contains the pyrimethamine-resistant Toxoplasma gondii (tg) dhfr/ts as a selectable marker cassette. See Figure 2—figure supplement 1 for the name and details of the construct pLIS0060. Target sequences for homologous recombination were PCR-amplified from P. berghei WT genomic DNA using primers specific for the 5' or 3' flanking regions of limp (see Supplementary file 2B for the sequence of the different primers). The PCR–amplified target sequences were cloned in plasmid pL0001 either upstream or downstream of the resistance cassette to allow for integration of the construct into the genomic target sequence by homologous recombination after digestion with Asp718I and NotI. Transfection into Fluo-frmg parasites (Mair et al., 2010), selection and cloning of mutant parasite lines were performed as described (Janse et al., 2006b). Deletion of limp was confirmed by diagnostic PCR (for primers see Supplementary file 2C) and Southern analysis of FIGE (field inversion gel electrophoresis)-separated chromosomes (Figure 2—figure supplement 1) with a probe recognising the 3' UTR of pbdhfr/ts. Absence of limp mRNA was determined by RT-PCR analysis (Figure 2—figure supplement 1; see Supplementary file 2C for primers used for RT-PCR). Two independently derived, cloned lines were used for phenotype analyses: 2091cl2m5 (Δlimp-a) and 2090cl2m6 (Δlimp-b), both in the Fluo-frmg background.
Generation of transgenic lines expressing GFP-, mCherry- and MYC-tagged LIMP
Request a detailed protocolIn situ C-terminal GFP tagging of limp was performed by single cross-over homologous recombination (see Figure 1—figure supplement 2 for details of the construct pLIS0079). Primers used to amplify the targeting region of limp are listed in Supplementary file 2B. The targeting region was cloned in frame with gfp. Linearised plasmid (AflII) was transfected into cl15cy1 parasites followed by limiting dilution cloning (Janse et al., 2006b), resulting in the transgenic line 2180cl1m4 (limp::gfp). Integration of the plasmid was confirmed by diagnostic PCR (for primers see Supplementary file 2C) and Southern analysis of FIGE-separated chromosomes using a probe for the 3' UTR of pbdhfr/ts (Figure 1—figure supplement 2). Transcription of the gfp fusion gene was confirmed by RT-PCR (Figure 1—figure supplement 2). Primers used for RT-PCR are listed in Supplementary file 2C.
To generate the parasite clone expressing N-terminally mCherry-tagged limp (C505.1), the mcherry ORF was integrated downstream of the signal peptide of limp. To ensure correct cleavage of the signal peptide, the sequence after the cleavage site was repeated downstream of the mcherry ORF. Endogenous 5' UTR and 3' UTR served as targeting regions for double homologous recombination (see Figure 4—figure supplement 2 for details of the plasmid construct pLIS0505). Integration of mcherry::limp into the limp locus of cl15cy1 parasites was confirmed via analytical PCR (Figure 4—figure supplement 2; for primers see Supplementary file 2C) of mcherry::limp parasites after limiting dilution cloning (Janse et al., 2006b).
C-terminal MYC tagging of limp was performed analogously to GFP tagging by single cross-over homologous recombination (See Figure 4—figure supplement 3 for details of the plasmid construct pLIS0472). Briefly, the limp::gfp construct was used as starting vector and gfp was replaced by a triple myc tag. Akin to limp::gfp, linearised limp::myc plasmid was transfected into cl15cy1 parasites followed by limiting dilution cloning (Janse et al., 2006b) producing clone C472.1. Correct integration of the plasmid was confirmed via PCR (Figure 4—figure supplement 3; for primers see Supplementary file 2C).
In vitro generation and purification of ookinetes for Western blot analysis
Request a detailed protocolBlood of an infected mouse was harvested by cardiac puncture and transferred to ookinete medium [250 mL RPMI 1640 supplemented with 25 mM HEPES and L-Glutamine (Gibco, #22400089); 12.5 mg hypoxanthine; 2.5 mL penicillin-streptomycin; 0.5 g NaHCO3; 5.12 mg xanthurenic acid; 20% FBS] at 19°C. After 20 hr, ookinetes were purified using a 63% Nycodenz cushion. After purification of ookinetes, uninfected red blood cells were removed by lysis with 0.17 M NH4Cl. The ookinete pellet was then incubated with RIPA buffer (50 mM Tris–HCl pH 7.5; 150 mM NaCl; 1% Triton X–100; 0.5% sodium deoxycholate; 0.1% SDS; 1 mM EDTA) for 1 hr on ice to lyse the parasites. Samples were then centrifuged for 30 min at 14,000 rpm at 4°C and Laemmli buffer was added to the supernatant.
Analysis of Δlimp blood-stage development
Request a detailed protocolNaive mice were infected intravenously (i.v.) with 104infected red blood cells (iRBCs) of either WT (Fluo-frmg) or Δlimp parasites. Total parasitaemia, female and male gametocytaemias were determined daily by FACS. Total parasitaemia was determined using the vital DNA dye Vybrant DyeCycle Ruby stain (Molecular Probes, #V10273). Given that both WT and Δlimp-a parasite lines express RFP in female gametocytes and GFP in male gametocytes, female gametocytaemias were calculated as RFP+ RBCs/total RBCs, while male gametocytaemias were calculated as GFP+ RBCs/total RBCs.
Ookinete formation assays
Request a detailed protocolOokinete formation assays were performed following published methods using gametocyte-enriched blood collected from mice treated with phenylhydrazine/NaCl (Beetsma et al., 1998). The ookinete conversion rate is defined as the percentage of female gametes that develop into mature ookinetes determined by counting female gametes and mature ookinetes in Giemsa-stained blood smears 16–18 hr after in vitro induction of gamete formation.
Oocyst and sporozoite production
Request a detailed protocolOocyst and sporozoite production of the mutant parasites was analysed by performing standard mosquito infections. Naive mice were infected intraperitoneally (IP) with 106 infected red blood cells (iRBCs) of each line. On days 4–5 p.i., mice were anaesthetised and Anopheles stephensi female mosquitoes allowed to feed for 30 min. Twenty-four hours after feeding, mosquitoes were anaesthetised by cold shock and unfed mosquitoes were removed. Oocyst and sporozoite numbers were counted at days 11–12 and 17–21 after mosquito infection, respectively. Oocysts were counted after mercurochrome staining. Sporozoites were counted in pools of 4–10 mosquitoes.
Transmission experiments
Request a detailed protocolTransmission of Δlimp-a parasites was assessed by injecting i.v. 3,500 salivary gland sporozoites dissected at day 20 p.i. into naive mice. Blood-stage parasitaemias were followed up to 14 days post-injection. Livers were extracted at 44 h.p.i. and parasite load determined by quantitative real-time PCR (qPCR) using specific primers for P. berghei ANKA 18S rRNA gene. Mouse hypoxanthine-guanine phosphoribosyltransferase (HPRT) was used as host tissue control gene. Primers used for qPCR are listed in Supplementary file 2A. Absolute number of mRNA copies was determined for each gene using standard curves.
In vitro sporozoite gliding motility assays
Request a detailed protocolWT (Fluo-frmg or cl15cy1), Δlimp-a, Δlimp-b and limp::gfp salivary gland sporozoites were dissected at days 20–21 p.i. and gliding motility assessed in a standard gliding assay (Liehl et al., 2010). Briefly, glass coverslips were coated overnight at RT with a 10 µg/mL suspension of 3D11 mouse anti-P. berghei circumsporozoite protein (CSP) monoclonal antibody (RRID:AB_2650479) (Yoshida et al., 1980). On the following day, 10,000–20,000 salivary gland sporozoites of each line were loaded per coverslip and incubated for 1 hr at 37°C, 5% CO2, in the presence of 10% FBS. In the case of limp::gfp, sporozoites were also pre-incubated for 1 hr on ice in the presence of rabbit polyclonal anti-GFP (Abcam, #ab6556; 10 µg/mL) (RRID:AB_305564) or control rabbit IgGs (Abcam, #ab37415; 10 µg/mL) (RRID:AB_2631996) to evaluate possible gliding blockade. Sporozoites were then fixed with 4% PFA/PBS and an anti-PbCSP immunofluorescence assay (IFA) was performed to detect CSP trails (see below for IFA details). Coverslips were analysed in a Leica DM5000B fluorescence microscope. Each sporozoite was categorised according to the number of trails it formed. Percentages of sporozoites in each category for each line were calculated as the ratio between the number of sporozoites in each category and the total number of sporozoites analysed. To perform live motility assays of haemolymph sporozoites, mosquitoes were dissected on days 15–16 p.i. To obtain haemolymph sporozoites, mosquitoes were cooled on ice for 20 min. After removing the last segment of the abdomen, the thorax was pierced with a glass pipette and the haemolymph was flushed out of the mosquito. Motility was assessed by imaging sporozoites in a Nunc MicroWell 96-well plate with optical bottom (Thermo Scientific) using an inverted Zeiss Axiovert 200M widefield microscope with an XBO75 xenon lamp, the AxioVision 4.7.2 software, a 25X objective (LCI Plan-NEOFLUAR ImmKorr NA 0.8, water) (all Zeiss) and a CoolSNAP HQ2 high-resolution CCD camera (Photometrics). Bright-field images were acquired every second for 3 min (181 frames per movie). The movement of sporozoites was assessed using ImageJ 1.44o software (imagej.nih.gov/ij). The imaged sporozoites were clustered into three different categories (Hegge et al., 2009): ‘continuously moving’ sporozoites (consistently gliding with a speed of at least 0.2 μm/s over a minimum of 90 s); ‘attached’ sporozoites (displaying circular gliding motility, but failing to meet the ‘moving’ requirements or not showing any circular gliding but attached at either one or both ends); and ‘floating’ sporozoites (not attached to the glass surface). The speed of continuously moving sporozoites was determined using the manual tracking plug-in of ImageJ. For the analyses of the movement of salivary gland sporozoites, mosquitos were dissected on days 17–25 p.i. Motility was evaluated as described above with the following changes: images were taken every 3 s for 5 min (101 frames per movie) and productively moving sporozoites moved for at least 100 s. To measure the front-to-rear distance of moving sporozoites, a straight line was drawn connecting both ends using the straight line tool of ImageJ.
In vitro sporozoite traversal, adhesion and invasion assays
Request a detailed protocolWT (Fluo-frmg or cl15cy1), Δlimp-a, Δlimp-b and limp::gfp salivary gland sporozoites were dissected at day 21 p.i. To test traversal of human hepatoma cells in vitro, 5,000 salivary gland sporozoites of each parasite line were added, in the presence of 0.5 mg/mL of Dextran, Tetramethylrhodamine (Molecular Probes, #D1817), onto 110,000 Huh7 cells plated 16–20 hr before in 24-well plates and incubated for 2 hr at 37°C, 5% CO2. Equivalent amounts of non-infected mosquito salivary gland debris were loaded as negative control. Cells were washed, trypsinised and analysed in a BD Biosciences FACSCalibur flow cytometer. Percentage of traversal was quantified as the ratio of Dextran-positive cells per live cells. To test the parasite capacity to adhere to and invade human hepatoma cells in vitro, 5,000 WT (Fluo-frmg or cl15cy1), Δlimp-a, Δlimp-b or limp::gfp salivary gland sporozoites were loaded onto 25,000 Huh7 cells plated 16–20 hr before in black-walled 96-well plates and incubated for 2 hr at 37°C, 5% CO2. In the case of limp::gfp, sporozoites were also pre-incubated for 1 hr on ice in the presence of rabbit polyclonal anti-GFP (Abcam, #ab6556; 10 µg/mL) (RRID:AB_305564) or control rabbit IgGs (Abcam, #ab37415; 10 µg/mL) (RRID:AB_2631996) to evaluate possible invasion blockade. Cells were then fixed with 4% PFA/PBS and a dual colour anti-PbCSP immunofluorescence assay was performed to distinguish between sporozoites that invaded from those that did not, following published methods (Rénia et al., 1988). Briefly, external sporozoites were detected before cell permeabilisation using a 10 µg/mL suspension of 3D11 mouse anti-PbCSP (RRID:AB_2650479) (Yoshida et al., 1980) followed by goat anti-mouse IgG-Cy3 (Jackson ImmunoResearch Laboratories, Inc., #115-166-003; 1:500) (RRID:AB_2338699). Cells were then permeabilised with 0.1% TritonX-100/PBS and total sporozoites detected by a second incubation with the same 3D11 mouse anti-PbCSP dilution followed by goat anti-mouse IgG-Alexa Fluor488 (Jackson ImmunoResearch Laboratories, Inc., #115-546-006; 1:500) (RRID:AB_2338860). Cells were imaged under a Zeiss Axiovert 200M fluorescence microscope. Adhesion was quantified as the ratio of imaged sporozoites per number of Huh7 cells in the same optical fields.
In vitro exoerythrocytic form (EEF) development assays
Request a detailed protocolWT (Fluo-frmg or cl15cy1), Δlimp-a, Δlimp-b and limp::gfp salivary gland sporozoites were dissected at day 21 p.i. and tested for their ability to transform into EEFs inside Huh7 cells in culture. Of each parasite line, 5,000 salivary gland sporozoites were loaded onto 10,000 Huh7 cells plated 16–20 hr before in black-walled 96-well plates and incubated for 45 hr at 37°C, 5% CO2. Cells were fixed with 4% PFA/PBS and an immunofluorescence (IFA) assay performed to detect parasite HSP70 and UIS4 (see below for IFA details). The area of cl15cy1 and limp::gfp EEFs were calculated based on HSP70 staining using ImageJ 1.47n software (imagej.nih.gov/ij).
Live imaging and immunofluorescence assays (IFAs) of blood stages, ookinetes and sporozoites
Request a detailed protocolLive imaging of transgenic limp::gfp parasites was done by retrieving ookinetes from mosquito blood meals at 16 h.p.i. To detect LIMP::GFP expression by IFA in blood stages, as well as in midgut and salivary gland sporozoites, mouse RBCs infected with limp::gfp parasites or dissected midgut and salivary gland sporozoites were stained with either rabbit polyclonal anti-GFP (Abcam, #ab6556; 1:500) (RRID:AB_305564), rabbit monoclonal anti-GFP (Life Technologies, #G10362) (RRID:AB_2536526), or mouse monoclonal anti-GFP (Abcam, #ab1218; 1:250) (RRID:AB_298911) as primary antibody. To detect mCherry::LIMP and LIMP::MYC, rabbit polyclonal anti-mCherry (Abcam, #ab183628) (RRID:AB_2650480) and mouse monoclonal anti-c-myc (Roche, #11667149001) (RRID:AB_390912) primary antibodies were used, respectively. As secondary antibody, goat anti-rabbit IgG-Alexa Fluor488 (Jackson ImmunoResearch Laboratories, Inc., #111-545-003; 1:500) (RRID:AB_2338046) or goat anti-mouse IgG-Alexa Fluor488 (Jackson ImmunoResearch Laboratories, Inc., #115-546-006; 1:500) (RRID:AB_2338860) was used. To detect CSP or TRAP in sporozoites, 3D11 mouse anti-PbCSP (RRID:AB_2650479) (Yoshida et al., 1980) (1:5,000) or rabbit polyclonal anti-PbTRAP repeats antiserum (RRID:AB_2650481) (Ejigiri et al., 2012) (1:1,000) were used. IFAs to detect HSP70 and UIS4 in in vitro-developed EEFs were done using parasite-specific 2E6 mouse monoclonal anti-PbHSP70 (RRID:AB_2650482) (Tsuji et al., 1994) at 18.75 µg/mL and goat polyclonal anti-PbUIS4 (SICGEN, #AB0042; 2 µg/mL) (RRID:AB_2333158/2333159), respectively, followed by donkey anti-mouse IgG-DyLight549 (Jackson ImmunoResearch Laboratories, Inc., #745-506-150; 1:500) (RRID:AB_2650483) and donkey anti-goat IgG-Alexa Fluor488 (Jackson ImmunoResearch Laboratories, Inc., #705-546-147; 1:500) (RRID:AB_2340430). For all IFAs, samples were fixed with 4% PFA/PBS for 10–60 min at RT, permeabilised (or not) with 0.1–0.2% Triton X-100/PBS for 10–20 min and blocked for 20–60 min at RT with 1–3% BSA/PBS. All antibody incubations were done in blocking solution for 45–60 min at RT and Hoechst-33342/PBS (1–5 μg/mL) or DRAQ5 (5 µM, Biostatus) was used to stain nuclei. Images were taken with Leica DM5000B and Zeiss Axiovert 200M fluorescence microscopes, as well as with a Leica TCS SP5 confocal microscope, and processed using ImageJ 1.47n software (imagej.nih.gov/ij).
Transmission electron microscopy (TEM) and immuno-gold EM of sporozoites
Request a detailed protocolInfected mosquito midguts and salivary glands were dissected on days 20–27 p.i and fixed for 3 hr at 4°C in 0.1 M cacodylate buffer, pH 7.4, containing 2.5% (v/v) glutaraldehyde. Following 1 hr of post-fixation with 1% (w/v) osmium tetroxide and 30 min of staining in 1% (w/v) uranyl acetate, samples were dehydrated in ethanol gradient (70–95–100%), transferred to propylene oxide and embedded in EPON resin. Semi-thin sections (300–400 nm) were stained with toluidine blue for light microscope evaluation. Ultra-thin sections (70 nm) were collected in Formvar-coated copper slot grids (AGAR Scientific) and then stained with 2% uranyl acetate and lead citrate (Reynolds recipe). For immuno-gold EM, ultra-thin sections (70 nm) collected in Formvar-coated Nickel 150 mesh grids were blocked for 30 min at RT with 0.8% BSA, 0.1% cold water fish skin gelatine, and incubated overnight at 4°C with rabbit polyclonal anti-GFP (Abcam, #ab6556; 1:50) (RRID:AB_305564). After a new blocking step of 15 min at RT, sections were incubated for 1 hr at RT with Protein A conjugated to 15 nm gold particles (obtained from Cell Microscopy Center, University Medical Center Utrecht, The Netherlands; 1:50). Sections were finally stained with 2% uranyl acetate and lead citrate (Reynolds recipe). Antibody and Protein A incubations were done in blocking solution. All grids were examined in a Hitachi H-7650 transmission electron microscope at 100kV acceleration.
Multiple sequence alignments
Request a detailed protocolProtein sequences in Figure 1B were retrieved from PlasmoDB (plasmodb.org) (RRID:SCR_013331) or from eupathdb.org (RRID:SCR_004512) for Figure 1—figure supplement 1. ClustalW alignments were performed at the EMBnet server (embnet.vital-it.ch/software/ClustalW.html) and shaded according to protein similarity levels with BOXSHADE 3.21 (www.ch.embnet.org/software/BOX_form.html) (RRID:SCR_007165).
Homology modelling of LIMP
Request a detailed protocolLIMP without signal peptide (I23-G110) was submitted to the QUARK online server (http://zhanglab.ccmb.med.umich.edu/QUARK/), an ab initio protein folding algorithm (Xu and Zhang, 2012). The model with the minimal TM score was chosen for all subsequent modelling experiments. To generate a model for LIMP::GFP, chain A of the GFP structure (PDB ID: 1GFL) was chosen, linked to LIMP using the Prime Module of the Schrödinger package (www.schroedinger.com) (RRID:SCR_014879) and used to develop a three-dimensional structure of LIMP::GFP. Analogously, mCherry (PDB ID: 2H5Q) was chosen for modelling mCherry::LIMP.
Molecular dynamics
Request a detailed protocolModelled LIMP, LIMP::GFP, mCherry::LIMP and LIMP::MYC were prepared for all-atom molecular dynamics (MD) simulations using the tleap program within the AMBER molecular dynamics package version 14 (Case et al., 2014) (http://ambermd.org) (RRID:SCR_014230); topology and parameters were generated using the ff99SBildn force field (Lindorff-Larsen et al., 2010); proteins were solvated using TIP3P water-model in truncated octahedron box type. Standard settings within PMEMD (Particle mesh Ewald molecular dynamics) were then used for the simulations following a two-step energy minimisation: minimisation while keeping restrain on the protein atoms (1,500 steps of steepest descent method), and all-atom minimisation (first 2,500 steps of steepest descent, next 1,000 steps of conjugate gradient). Minimised systems were then gradually heated (0 to 298 Kelvin in 100 picoseconds) using canonical ensemble (NVT). In the next step, we equilibrated pre-heated system in isothermal–isobaric ensemble (NPT) at 298 Kelvin: Berendsen temperature coupling and a constant pressure of 1 atm with isotropic molecule-based scaling was used in the equilibration. To reduce simulation run time, the SHAKE algorithm was applied to fix all covalent bonds containing hydrogen atoms. A 10 Å cut-off was applied to treat nonbonding interactions such as short-range electrostatics and van-der-Waals interactions, while the particle-mesh-Ewald (PME) method was used for long-range electrostatic interactions. Simulations were carried out with periodic boundary condition in NPT ensemble for 100 ns. The analyses of MD simulations were carried out by CPPTRAJ module of AMBER 14. Visual Molecular Dynamics (VMD) (RRID:SCR_001820) (Humphrey et al., 1996) and PyMOL (www.pymol.org) (RRID:SCR_000305) was used for visualisation.
Statistical methods
Request a detailed protocolStatistical analyses were performed using Prism software package 5 or higher (GraphPad Software) (RRID:SCR_002798).
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Article and author information
Author details
Funding
Fundação para a Ciência e a Tecnologia (PTDC/BIA-BCM/105610/2008)
- Gunnar R Mair
Fundação para a Ciência e a Tecnologia (PTDC/SAU-MIC/122082/2010)
- Gunnar R Mair
Fundação para a Ciência e a Tecnologia (SFRH/BD/63849/2009)
- Jorge M Santos
Fundação para a Ciência e a Tecnologia (BPD/81953/2011)
- Vanessa Zuzarte-Luís
Horizon 2020 Framework Programme (Marie Sklodowska-Curie grant agreement No 660211)
- Saskia Egarter
Horizon 2020 Framework Programme (ERC-SG 281719)
- Friedrich Frischknecht
Human Frontier Science Program (RGY007½011)
- Friedrich Frischknecht
Chica and Heinz Schaller Foundation
- Friedrich Frischknecht
Seventh Framework Programme (EviMalar)
- Friedrich Frischknecht
The funders had no role in study design, data collection and interpretation, or the decision to submit the work for publication.
Acknowledgements
We would like to thank Ana Guerreiro, Ana Parreira and Fernanda Baptista (iMM Lisboa), as well as Jai Ramesar and Johannes Kroeze (LMRG, LUMC) for management and experimental support; Leonor Pinho and Miriam Reinig for mosquito production; Drs. Céline Carret and António Mendes (iMM Lisboa) for technical advice; Dr. Photini Sinnis (JHMRI, JHSPH, USA) for providing the anti-PbTRAP antiserum; Dr. Erin Tranfield (IGC EM Facility, Portugal) for technical and intellectual input during EM experiments; and access to bwGRiD (http://www.bw-grid.de), member of the German D-Grid initiative, funded by the Ministry for Education and Research (Bundesministerium für Bildung und Forschung) and the Ministry for Science, Research and Arts Baden-Wuerttemberg (Ministerium für Wissenschaft, Forschung und Kunst Baden-Württemberg).
Ethics
Animal experimentation: In Instituto de Medicina Molecular (iMM, Lisbon, Portugal), animal experimentation protocols were approved by the iMM Animal Ethics Committee (under authorisation AEC_2010_018_GM_Rdt_General_IMM) and the Portuguese authorities (Direção Geral de Alimentação e Veterinária). Animal experiments performed in Leiden University Medical Center (LUMC, Leiden, The Netherlands) were approved by the Animal Experiments Committee of the Leiden University Medical Center (DEC 10099; 12042; 12120). At the University of Heidelberg Medical School (Heidelberg, Germany) animal work was approved by the German authorities (Regierungspräsidium Karlsruhe; 35-9185.81/G-266/16) and performed in compliance with FELASA guidelines and regulations. All animal work was in accordance with EU regulation. Animals used were female BALB/c, OF-1 and NMRI mice (6-8 weeks old) bred at Charles River or Janvier, France.
Copyright
© 2017, Santos et al.
This article is distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use and redistribution provided that the original author and source are credited.
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