Expression Profiling of Plasmodium berghei HSP70 Genes for Generation of Bright Red Fluorescent Parasites

Live cell imaging of recombinant malarial parasites encoding fluorescent probes provides critical insights into parasite-host interactions and life cycle progression. In this study, we generated a red fluorescent line of the murine malarial parasite Plasmodium berghei. To allow constitutive and abundant expression of the mCherry protein we profiled expression of all members of the P. berghei heat shock protein 70 (HSP70) family. We identified PbHSP70/1, an invariant ortholog of Plasmodium falciparum HSP70-1, as the protein with the highest expression levels during Plasmodium blood, mosquito, and liver infection. Stable allelic insertion of a mCherry expression cassette into the PbHsp70/1 locus created constitutive red fluorescent P. berghei lines, termed Pbred. We show that these parasites can be used for live imaging of infected host cells and organs, including hepatocytes, erythrocytes, and whole Anopheles mosquitoes. Quantification of the fluorescence intensity of several Pbred parasite stages revealed significantly enhanced signal intensities in comparison to GFP expressed under the control of the constitutive EF1alpha promoter. We propose that systematic transcript profiling permits generation of reporter parasites, such as the Pbred lines described herein.


Introduction
Malaria is caused by blood infection of the obligate intracellular parasite Plasmodium, single cell eukaryotes that follow a complex developmental program during life cycle progression.Although many aspects of the parasite life cycle are known since decades, previously unrecognized aspects of the clinically silent and diagnostically inaccessible pre-erythrocytic phase, such as cell traversal prior to productive invasion [1], intradermal migration of sporozoites [2], and formation of merosomes as the final step in liver stage maturation [3], have profoundly transformed our understanding of Plasmodium biology.These observations were possible because generation of a bright green fluorescent sporozoite line, CSP::GFP [4], permitted live imaging of sporozoite-infected animals.
Stable transgenic expression of fluorescent proteins is an established strategy in Plasmodium parasites and is an invaluable tool for in vivo studies on temporal and spatial gene expression.In addition, fluorescent parasites can serve as reference lines for biological studies.The fluorescent proteins of choice include green fluorescent protein (GFP) from the jellyfish Aequorea victoria [4][5][6], red fluorescent protein (RFP) and its improved version, RedStar [7,8], and the red fluorescent protein mCherry [9][10][11].The first GFP-expressing Plasmodium line was generated by stable integration of a dihydrofolate reductase/thymidylate synthase (DHFR-TS) -GFP fusion protein into the P. berghei genome [12].Due to the low promoter activity, fluorescence was relatively weak, prompting subsequent strategies to search for strong, albeit stage-specific, promoters [4,8].This limitation was partially overcome by generation of fluorescent parasites that express GFP under control of the elongation factor 1 alpha (EF1a) promoter, resulting in constitutive, but only moderate, fluorescence throughout the parasite life cycle [6].
In this study, we aimed at generating transgenic, constitutive, red fluorescent P. berghei parasites towards robust live cell imaging throughout the entire Plasmodium life cycle.For this purpose, we focused on members of the heat shock protein 70 (HSP70) family, because they are ubiquitous, typically abundant, and likely to perform important functions in Plasmodium parasites [13][14][15].In general, HSP70 members are ATPases that tightly bind peptide substrates in their ADP-bound state in order to prevent misfolding or aggregation of the polypeptide substrate, hence the term 'chaperones'.Plasmodium species encode at least four conserved HSP70 members that localize to various compartments in the parasite and likely fulfill distinct chaperone functions (Fig. 1).
A Toxoplasma gondii ortholog, TgHSP70.1 (TGME49_073760; gi: 3850199) was readily identified (Fig. 1A).Intriguingly, posttranscriptional regulation and allelic variants of this protein were implicated in T. gondii virulence [28].Together, these findings indicate that the HSP70/1 promoter is a strong candidate for transgenic expression of reporter proteins.The structurally related and exported protein PfHsp70-x (PF3D7_0831700; MAL7P1.228) is present only in P. falciparum and the related parasite P. reichenowi, where it fulfills a specialized role in remodeling the host erythrocyte [29], and, hence, could not be included in this study (Tab.S1).
We finally included the Hsp70/Hsp90 organizing protein (HOP) in our expression analysis.HOP was originally identified as a 60 kDa stress-related protein that forms a complex with HSP70 and HSP90 [33] and contributes to efficient chaperone cooperation.Initial characterization of PfHOP (PF3D7_1434300; PF14_0324) showed a cytoplasmic localization and indicated that the protein might associate with PfHSP70-1 [34].PbHOP (PBANKA_101050; gi: 68071103) and TgHOP (TGME49_052220; gi: 237840065) are readily identified based on high sequence conservation (Tab.S1).
In this study, we performed systematic transcript profiling of the P. berghei HSP70 family throughout the entire Plasmodium life cycle and, thereby, identified Hsp70/1 as a candidate promoter region for robust, constitutive, and high level expression of a red fluorescent reporter protein for live cell imaging applications.

Expression Profiling of P. berghei HSP70 Transcripts
We initiated our analysis by systematic quantitative RT PCR (qRT PCR) profiling of HSP70 and HOP mRNAs in different life cycle stages of the murine malarial parasite P. berghei (Fig. 2).To this end, we isolated RNAs from (i) gradient-purified late blood stages, so-called schizonts, (ii) enriched gametocytes by drug treatment of P. berghei-infected mice, (iii) cultured ookinetes, (iv) sporozoites liberated from infected Anopheles salivary glands, and cultured sporozoite-infected hepatoma cells, representing (v) early (24 h) and (vi) late (48 h) liver stages.Profiling of steady-state transcript abundance by qRT PCR using gene-specific primer pairs and normalization to GFP expressed under the control of elongation factor 1 alpha (EF1a) revealed robust expression for all transcripts analyzed (Fig. 2).
In all life cycle stages examined, PbHSP70/1 was the most abundant transcript compared to all other HSP70 members tested.Expression levels were also typically 2-10-fold higher than the GFP reference transcript.This difference was most apparent in ookinetes, schizonts/merozoites, and late liver stages, indicating substantially enhanced signal intensity as compared to EF1a, making PbHSP70/1 the prime candidate to drive reporter gene expression.
PbHSP70/2/BIP/GRP-78 steady-state levels fluctuated substantially depending on the life cycle phase, ranging from very low (,100 fold reduced) expression in sporozoites to high (,10 fold upregulated) levels in schizonts (Fig. 2).The PbHSP70/2 expression pattern highlights the importance of profiling multiple life cycle stages and indicates differential importance of protein refolding in the ER, and perhaps the organelle as a whole, during Plasmodium life cycle progression.
Transcripts of the two organelle-imported HSP70-members, PbHSP70/3 and PbHSP70/y, were stably expressed throughout the life cycle, but never exceeded the levels of the GFP reference transcripts (Fig. 2).Finally, PbHOP expression resembled PbHSP70/1 expression, albeit at a substantially lower level (Fig. 2).Together, this analysis identified the PbHSP70/1 promoter as the best candidate to develop a robust reporter parasite with enhanced fluorescence.

Generation of Pbred Parasites
We next created a P. berghei targeting plasmid that would permit stable integration of mCherry under the control of the PbHSP70/1 promoter (Fig. 3).To this end, we amplified 2.2 kb of the 59 untranslated region (UTR) of PbHSP70/1 as the respective promoter sequence and fused it upstream of the mCherry open reading frame, followed by the heterologous 39UTR of the P. berghei dihydrofolate reductase/thymidylate synthase (DHFR/TS).Upon linearization in the 59UTR the targeting plasmid is integrated via a single cross-over event (Fig. 3A).The resulting allelic diploid contains a 59 copy with the desired mCherry expression cassette and a 39 copy that corresponds to the endogenous PbHSP70/1 locus.
We performed transfections into two P. berghei strains, namely wild-type (WT) parasites (strain ANKA) and clone 507 [6], a WTlike parasite (strain ANKA) that expresses GFP under the control of the constitutive EF1a promoter generating Pbred clone ANKA (Pbred c ANKA ) and Pbred clone 507 (Pbred c 507 ), respectively.Generation of the Pbred c 507 parasite line, emitting GFP controlled by the EF1a promoter and mCherry driven under the Hsp70/1 promoter, allowed us to quantify and compare both fluorescent signals in individual parasites.
Genotyping by diagnostic PCR revealed the predicted sitespecific integration in both recipient parasites (Fig. 3B).The resulting parasite lines were cloned in vivo by limiting dilutions, resulting in two clonal Pbred c ANKA and Pbred c 507 parasite populations.

Pbred Parasites Develop Normally throughout the Plasmodium Life Cycle
Next, we monitored blood infection in outbred NMRI mice to ascertain that the expression cassette does not interfere with parasite growth in vivo (Fig. 4).Monitoring of parasitemia after intravenous injection of 1,000 infected erythrocytes revealed that parasite proliferation and population expansion of both Pbred clones are indistinguishable from wild-type (WT) parasites during blood stage development.
We next analyzed mosquito stage development of the Pbred parasites by determination of salivary gland sporozoite numbers in infected A. stephensi mosquitoes (Fig. S1).Sporozoite numbers of Pbred c 507 and WT parasites were indistinguishable, indicating normal life cycle progression in the mosquito host.Furthermore, natural transmission of the Pbred c 507 parasite line was tested by a so-called bite-back experiment.C57/Bl6 mice where exposed to WT-or Pbred c 507 -infected mosquitoes and parasitemia was tested daily by microscopic examination of Giemsa-stained blood smears.In all animals tested, blood stage parasites where first detected three days after sporozoite exposure (data not shown).This finding indicates normal liver stage development of Pbred c 507 parasites.Together, we conclude that Pbred parasites are suitable as a P. berghei reference line, since replication, viability, and infectivity are indistinguishable from WT parasites.

Live-cell Imaging and Quantitative Fluorescence Analysis of Pbred Parasites
We initiated our imaging analysis with infected erythrocytes (Fig. 5).Fluorescence microscopy of whole blood ex vivo revealed bright red fluorescence throughout all asexual blood stage parasites and gametocytes (Fig. 5A).Fluorescence intensity appeared uniform in all stages and permits classical morphological distinction of different parasite stages based on the combination of the strong cytoplasmic red fluorescence and the blue fluorescent nuclear signal obtained with Hoechst 33528.In comparison, the GFP fluorescence signal was relatively low, and virtually undetectable in young parasites, i.e. ring stages (Fig. 5A).Quantitative comparison of the mCherry and GFP signals revealed significant differences in ring stages and trophozoites and overall brighter signals for both fluorescent proteins in gametocytes (Fig. 5B).
We next analyzed parasite development in the mosquito vector (Fig. 6).Mosquito infection with Pbred c 507 parasites could readily be identified in the midgut and salivary glands of live mosquitoes, because of the strong red fluorescence of the respective parasite populations in these organs (Fig. 6A).This finding prompted us to explore whether we could image individual sporozoites in whole mosquitoes, as previously achieved with transgenic parasites that express GFP or mCherry under the control of the circumsporozoite protein (CSP) promoter [35,36].Intriguingly, we could readily capture individual bright red fluorescent hemocoel sporozoites in wing veins and the maxillary palps of infected mosquitoes (Fig. 6B).The corresponding GFP signal was typically too weak for live imaging, as illustrated for hemocoel sporozoites in a wing vein.
Dissection of Pbred-infected mosquitoes at various time points recovered bright red fluorescent ookinetes, infected midguts, single midgut-associated oocysts, and individual salivary gland sporozo-ites, respectively (Fig. 7).All parasite stages were amenable to live cell imaging and displayed strong red fluorescence signals, as expected from the whole mosquito imaging.
We finally captured the pre-erythrocytic, liver stage development phase of the life cycle (Fig. 8).Intra-hepatic maturation was monitored by in vitro infection of human hepatoma cells Huh7 with Pbred c 507 sporozoites.Strong red fluorescence illuminating the parasite cytoplasm of hepatic stages and merosomes, in good agreement with mCherry being a soluble protein that lights up the cytoplasm in all parasite stages described.
In order to compare both fluorophores in a quantitative manner, we performed fluorescence quantification for ookinetes, sporozoites and liver stages of Pbred c 507 parasites (Fig. 9).When we analysed the distribution of the brightness of all pixels for representative parasite stages we detected a broader distribution of high values (Fig. 9A) and significantly higher mean intensities (Fig. 9B) for mCherry as compared to GFP signals in all stages tested.
Together, live cell imaging of the transgene Pbred parasite confirmed that mCherry, expression under the Hsp70/1 promoter, results in strong and stable intensity of red fluorescence throughout the entire life cycle as predicted by initial gene expression analysis.

Discussion
In this study, we developed red fluorescent reporter parasite lines, Pbred, termed Pbred c 507 and Pbred c ANKA , displaying strong and robust fluorescence throughout the entire Plasmodium life cycle.We identified a constitutive strong promoter to express mCherry by gene expression analysis of Hsp70 proteins via quantitative RT-PCR.This analysis revealed PbHsp70/1 as the most abundant gene transcript throughout the parasite life cycle, closely resembling constitutive expression of the human ortholog Hsc70.Transcript normalization to GFP expressed under the EF1a promoter allowed us to select a promoter that is consistently stronger and most likely appropriate to drive robust and enhanced fluorescence.While we have not addressed HSP70/1 function by experimental genetics, we consider it highly likely that the gene  performs critical roles in all life cycle stages and will be refractory to targeted gene deletion.
All other members of the Hsp70 family, PbHSP70/2, PbHSP70/ 3, PbHSP/y and PbHOP exhibited lower expression levels, in agreement with their organelle targeting or complex organizing role.Intriguingly, expression of the ER-resident PbHSP70/2 fluctuated substantially.This expression pattern contrasts with the HSP70 members in mitochondria and the apicoplast.Previous work showed that stable fluorescent organelle labeling is feasible [37][38][39].In agreement with our PbHSP70/3 and PbHSP/y expression data, there was a good correlation of organelle and parasite sizes for apicoplast and mitochondria [38,39].It will be interesting to visualize the ER throughout the life cycle and to study whether this organelle expands and contracts, as indicated by the differential expression of PbHSP70/2.The Pbred parasite lines were engineered by fusion of mCherry with the PbHSP70/1 promoter sequence and stable allelic integration by a single crossover event into the PbHSP70/1 locus.Phenotypic analysis of the Pbred clones verified that transgenic expression of the fluorescent protein mCherry did not alter the fitness of the parasite as compared to wild type parasites.We used the double fluorescent Pbred c 507 parasite line to quantify mCherry expressed under the Hsp70/1 promoter with GFP expressed under the EF1a promoter [6].Fluorescence quantitation of diverse Pbred c 507 parasite stages, revealed significant enhanced mCherry signal throughout the life cycle as compared to GFP fluorescence.Our quantification is consistent with earlier reports of bright GFP expression in ookinetes and sporozoites [40,41].The quantum yield of GFP (QY = 0.60) and its excitation coefficient (e = 55,000) are two-fold higher than of mCherry (QY = 0.08, e = 26,000) [9] (ttable S3).Nevertheless, the mCherry fluorescence of Pbred c 507 was between three to seven-fold brighter than the GFP signals.This observation is most likely due to the strong promoter activity of HSP70/1 and is in good agreement with our gene expression analysis.Despite lower intrinsic brightness of mCherry (0.06) as compared to EGFP (1.0) or dtTomato (1.44) advantages of mCherry include fast protein maturation (15 min) and enhanced photo-stability [9].Accordingly, mCherry is particularly suited for in vitro and in vivo imaging of Plasmodium parasites [11].Therefore, the Pbred clones can be used as reference strains alone or in combination with constitutive green fluorescent parasites [42].Applications include, but are not limited to, growth competition assays in mice and mosquitoes, cross-fertilization experiments, and establishing kinetics of organ colonization.It is important to note that the expression cassette described herein can also be readily adapted to fluorescent labeling of mutant parasite lines generated by targeted gene deletion [42] and be used for rapid fluorescenceassisted cell sorting (FACS) of recombinant parasites [43].A recent related example is comparative live cell imaging of wild type and hsp20(-) sporozoites, which revealed a specific role for the small heat shock protein 20 (HSP20) in fast, continuous sporozoite locomotion and natural malaria transmission [44].
Fluorescent reporter parasites are important tools to study the complex developmental program, parasite/host cross talk, and parasite population dynamics throughout the Plasmodium life cycle.Robust and continuous monitoring of live parasites during processes such as host cell invasion, tissue transmigration, intracellular growth, proliferation, and host cell egress in the mammalian and invertebrate hosts are expected to expand our insights into fundamental aspects of parasite stage conversion and adaptation to new environments.Similarly, capturing of innate defense responses and targeted inactivation by the adaptive immune system will generate important mechanistic insights into the molecular mechanisms of host susceptibility and refractoriness, of naturally acquired immunity, and of vaccine-induced protection.Since effector cells in Plasmodium hosts are typically labeled by transgenic GFP expression, mCherry-expressing parasites provide the matching partners for capturing pathogen-host cell interactions at single cell resolution.

Ethics Statement
All animal work was conducted in accordance with the German 'Tierschutzgesetz in der Fassung vom 18. Mai 2006 (BGBl.I S. 1207)', which implements the directive 86/609/EEC from the European Union and the European Convention for the protection of vertebrate animals used for experimental and other scientific purposes.The protocol was approved by the ethics committee of MPI-IB and the Berlin state authorities (LAGeSo Reg# G0469/ 09).Experimental Animals, Parasites, and Cell Lines Female NMRI and C57Bl/6 mice were from Charles River Laboratories.We used P. berghei ANKA and isogenic parasites expressing GFP under the control of the EF1a promoter [6] as recipient parasites for transfection.Hepatoma cells (HuH7) were cultured as described [10].

Gene Expression Profiling
For qRT-PCR analyses, mRNA was isolated from schizontenriched blood stages (merozoites), gametocytes, ookinetes, sporozoites, and 24-and 48-hour liver stages of GFP-expressing P. berghei wild-type (WT) parasites (strain ANKA) [6] using the RNeasy kit (Quiagen).After DNase treatment, the mRNA of each sample was reversely transcribed to cDNA using oligo-dT primers of RETROScript kit (Ambion).Quantitative real time RT-PCR was performed on cDNA preparations as described [10] using the StepOnePlus TM Real-Time PCR System and Power SYBRH Green PCR Master Mix (Applied Biosystems) according to the manufacturer's instructions.qRT PCR was performed in duplicates of one mRNA pool per sample and the whole series was reproduced in a second and third independent experiment.Primers are listed in Table S1.Relative transcript abundance was determined using the 2 2DDCt method (Applied Biosystems).Expression data was normalized to the constitutive GFP gene expression of P. berghei ANKA GFP parasites [6].

Generation of Fluorescent Pbred Parasites
In order to obtain strong mCherry expression throughout the complete P. berghei life cycle, we chose the promoter sequence of the constitutive highly expressed gene HSP70/1 (PBANKA_071190) protein to drive fluorescent mCherry protein expression.An HSP70/1 59 region of 2,220 bp was selected as promoter sequence and amplified from gDNA using primers HSP70_for and HSP70_rev.The resulting fragment was cloned via EcoRI and BamHI restriction sites into a P. berghei targeting plasmid, termed pSE61 (kindly provided by Dr. Sabine Engelmann).Subsequently, mCherry was amplified from the plasmid B3D+mCherry [10] using primers mCherry_for-BamHI and mCherry_rev_SpeI and cloned via BamHI and SpeI downstream of the 59 promoter sequence.mCherry transcript stability was facilitated by cloning of the 39 UTR of P. berghei dihydrofolate reductase/thymidylate synthase (DHFR/TS) downstream of mCherry.The final plasmid, pHSP70/1::mCherry, was used for P. berghei transfection [6].Two independent parasite transfections with clone 507 and clone ANKA GFP were done with 10 mg each of BstBI-linearized pHSP70/1::mCherry and gradient-purified schizonts of either green fluorescent ANKA parasites (cl507) [6] or WT ANKA parasites using the NucleofactorH device (Amaxa).Positive selection of transgene parasites was performed by oral pyrimethamine in the drinking water.Clonal parasite lines were obtained by limiting dilution series and intravenous injection into 6 recipient NMRI mice.Genotyping of clonal parasite lines was performed by diagnostic PCRs using specific primers THsp70_1 for/T16mCherry_rev and THsp70_1rev/pSE61_for detecting 59 and 39 integration, in the desired clones, respectively.All primer sequences are listed in Table S2.

Phenotypical Analysis during the Plasmodium Life Cycle in vivo
Blood stage development was analyzed in vivo in asynchronous infections using NMRI mice.Gametocyte differentiation and exflagellation of microgametes were detected in mice before mosquito feedings.Anopheles stephensi mosquito rearing and maintenance was carried out under a 14 h light/10 h dark cycle, 75% humidity and at 28uC.Once infected, Anopheles mosquitoes were kept at 80% humidity and 20uC.Sporozoite populations were separated and analyzed as described previously [45].Briefly, for determination of sporozoite development, mosquitoes were dissected from salivary glands at day 17 after feeding and sporozoite numbers determined.For determination of sporozoite infectivity four C57Bl/6 mice were exposed to 15 Pbred and WT infected mosquitoes.Pre patency period was determined by daily microscopic examination of Giemsa-stained blood smears.Asexual blood-stage development was investigated by infection of mice with intravenous injection of 1,000 infected erythrocytes.Parasitemia of recipient mice (n = 5 for Pbred c 507 ; n = 3 for Pbred c ANKA ) was monitored daily by examination of Giemsa-stained blood smears.
Live Cell Imaging of Pbred c 507 throughout the Plasmodium Life Cycle Mixed blood stage parasites were obtained by tail vein puncture of infected NMRI mice and imaged live in 37uC pre-warmed RPMI media on ConcavalinA coated glass cover slips.Ookinetes were cultured for 18 h and purified as described [46].Imaging was done in complete ookinete medium.All mosquito stages were dissected in 3% BSA RPMI media and placed in dissecting media on Vaseline sealed glass slides.Parasite liver stage development was monitored in human hepatoma cells (Huh.7).Cells were infected with 20.000 salivary gland sporozoites in DMEM medium and microscopically observed at indicated time points after infection.Parasite and host cell DNA was visualized with Hoechst 33342 (1:1,000 dilution; Molecular Probes) for 10 min.Live cell imaging was performed using the Apoptome Imager Z2 Microscope (Zeiss).Representative parasite images where taken using the 206 and 636objective.Sporozoite colonized proboscis and mosquito wing veins were observed using the 406objective.Whole mosquito sample pictures were taken with a fluorescent binocular microscope (Leica).

Quantitative Image Analysis
Live cell imaging of Pbred c 507 parasite stages was performed by wide-field fluorescence microscopy using the Apoptome Imager Z2 Microscope (Zeiss) equipped with an AxioCam (Zeiss).For GFP detection filter sets 38 (Zeiss) with excitation BP 470/40 and emission BP 525/50, and for mCherry detection, filter set 43 (Zeiss) with excitation BP 550/25 were used.Whole ex vivo blood samples were imaged in 37uC pre-warmed RPMI media.Images were captured with the Plan-Apochromat 636/1,40 oil objective (Zeiss), and GFP and mCherry signals were measured using same exposure settings of 20 ms to allow direct comparison.To quantify the fluorescence intensity we determined grey values over the parasite area using the software ImageJ and presented our results as the mean of intensity values per pixel.The distribution of grey values in each channel was measured over the parasite area by drawing a ''mask'', encircling the parasite, and the cumulative grey values and corresponding pixel numbers calculated with the histogram function of ImageJ.To compare fluorescence intensities of GFP and mCherry between all parasite stages, the mean of grey values (6 S.E.M.) was calculated.Statistical tests were computed with GraphPad Prism 5.0.Statistical significance for fluorescence intensities was determined using the two-tailed t-test.A P value of ,0.05 was taken as significant.

Figure 3 .
Figure 3. Generation of Pbred parasites.(A) Integration strategy to generate Pbred parasites.The PbHSP70/1 genomic locus was targeted with an integration plasmid containing the 59 region flanking the HSP70/1 ORF (black box), the mCherry open reading frame (red box) and the 39 region of the PbDHFR, followed by the Tgdhfr/ts cassette as positive selectable marker.Upon linearization of the plasmid with BstBI, integration is expected to lead to allele duplication, resulting in mCherry expression under the PbHSP70/1 promoter and an adjacent PbHSP70/1 wild-type copy.Integration and wild type-specific test primer combinations and expected fragments are indicated.(B) Genotyping of two clonal Pbred parasite lines, Pbred c 507 and Pbred c ANKA .Confirmation of the predicted integration is achieved by PCR analysis using primer combinations (59UTR and 39 UTR), which only amplify a signal from the recombinant locus.A wild type-specific primer combination (WT) confirms the absence of residual wild type parasites in the clonal Pbred populations.doi:10.1371/journal.pone.0072771.g003

Figure 5 .Figure 6 .
Figure 5. Live imaging and fluorescence quantification of Pbred during blood infection.(A) Live cell imaging of Pbred c 507infected erythrocytes during blood stage development.Representative differential interference contrast DIC (left) and live fluorescent images for mCherry (center) and the green fluorescent proteins GFP (right) of Pbred-infected erythrocytes at different stages of development are shown.Nuclear stains (Hoechst) are visualized as merge in the DIC images.Life cycle stages are indicated on the left.Scale bars, 5 mm.(B) Quantitative analysis of mCherry (red) and GFP (green) fluorescence in different blood stages.Fluorescence intensities are presented in mean of grey values (6 S.E.M.) for rings, trophozoites and gametocytes.*, P,0.05 (students t-test).doi:10.1371/journal.pone.0072771.g005

Figure 7 .
Figure 7. Live cell imaging of Pbred during mosquito infection.Representative live cell images of Pbred c 507 development inside the Anopheles vector.Presented are DIC images in combination with nuclear stain (Hoechst; left) and fluorescent images for mCherry (center) and GFP (right).Life cycle stages are indicated on the left.Scale bars, 5 mm for ookinete and sporozoite, and 10 mm for oocyst, respectively.doi:10.1371/journal.pone.0072771.g007

Figure 8 .
Figure 8. Live cell imaging of Pbred parasites during infection of cultured hepatoma cells.Representative live cell images of Pbred c 507 -infected hepatoma cells at different stages of maturation.Presented are DIC images in combination with nuclear stain (Hoechst; left) and fluorescent images for mCherry (center) and GFP (right).Time points after sporozoite infection are indicated on the left.Scale bars, 10 mm for 24 h and 48 h time points and merosomes, and 20 mm for 72 h time points, respectively.doi:10.1371/journal.pone.0072771.g008