Figures
Abstract
Background
Trypanosoma cruzi is a parasitic protist that causes Chagas disease, which is prevalent in Latin America. Because of the unavailability of an effective drug or vaccine, and because about 8 million people are infected with the parasite worldwide, the development of novel drugs demands urgent attention. T. cruzi infects a wide variety of mammalian nucleated cells, with a preference for myocardial cells. Non-dividing trypomastigotes in the bloodstream infect host cells where they are transformed into replication-capable amastigotes. The amastigotes revert to trypomastigotes (trypomastigogenesis) before being shed out of the host cells. Although trypomastigote transformation is an essential process for the parasite, the molecular mechanisms underlying this process have not yet been clarified, mainly because of the lack of an assay system to induce trypomastigogenesis in vitro.
Methodology/Principal Findings
Cultivation of amastigotes in a transformation medium composed of 80% RPMI-1640 and 20% Grace’s Insect Medium mediated their transformation into trypomastigotes. Grace’s Insect Medium alone also induced trypomastigogenesis. Furthermore, trypomastigogenesis was induced more efficiently in the presence of fetal bovine serum. Trypomastigotes derived from in vitro trypomastigogenesis were able to infect mammalian host cells as efficiently as tissue-culture-derived trypomastigotes (TCT) and expressed a marker protein for TCT. Using this assay system, we demonstrated that T. cruzi inositol 1,4,5-trisphosphate receptor (TcIP3R)—an intracellular Ca2+ channel and a key molecule involved in Ca2+ signaling in the parasite—is important for the transformation process.
Citation: Hashimoto M, Morales J, Uemura H, Mikoshiba K, Nara T (2015) A Novel Method for Inducing Amastigote-To-Trypomastigote Transformation In Vitro in Trypanosoma cruzi Reveals the Importance of Inositol 1,4,5-Trisphosphate Receptor. PLoS ONE 10(8): e0135726. https://doi.org/10.1371/journal.pone.0135726
Editor: Juan Carlos Pizarro, Tulane University, UNITED STATES
Received: June 1, 2015; Accepted: July 24, 2015; Published: August 12, 2015
Copyright: © 2015 Hashimoto et al. This is an open access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are credited
Data Availability: All relevant data are within the paper and its Supporting Information files.
Funding: This work was supported by JSPS KAKENHI Grant Numbers 15K08452 (to MH), 24390102 (to TN) (https://www.jsps.go.jp/english/index.html). This work was supported by The Pharmacological Reserch Foundation, Tokyo (to MH) (http://www.disclo-koeki.org/08a/00994/1.pdf#search='%E5%85%AC%E7%9B%8A%E8%B2%A1%E5%9B%A3%E6%B3%95%E4%BA%BA+%E8%96%AC%E7%90%86%E7%A0%94%E7%A9%B6%E4%BC%9A'). This work was supported in part by the Foundation of Strategic Research Projects in Private Universities (S1201013) from the Ministry of Education, Culture, Sport, Science, and Technology, Japan (to TN) (http://www.mext.go.jp/english/). The funders had no role in study design, data collection and analysis, decision to publish, or preparation of the manuscript.
Competing interests: The authors have declared that no competing interests exist.
Introduction
Trypanosoma cruzi is a parasitic protist that causes Chagas disease, which is prevalent in Latin America [1]. The life cycle of T. cruzi is complex and consists of two phases: insect and mammalian stages. Either stage includes replicative and infective (non-replicative) forms. In the insect stage, a replicative form called epimastigote dwells in the mid-gut of blood-sucking reduviid insects and transforms into the metacyclic trypomastigote (metacyclogenesis), which can infect mammalian hosts. In the mammalian stage, the metacyclic trypomastigote invades a wide variety of nucleated cells and transforms into an amastigote, which replicates in the host cell cytoplasm by binary fission. After successive rounds of replication, the amastigote transforms back into a trypomastigote, which disrupts the host cell and is released into the circulation, from where it can propagate the infection.
Transformation between the developmental stages is essential for parasite survival. Identification of the key factors that trigger transformation is important not only for understanding the nature of the parasite but also for developing anti-parasitic drugs. Among the transformation steps, the mechanisms underlying metacyclogenesis have been extensively studied. Metacyclogenesis is induced by free fatty acids [2], cAMP [3–5], and depletion of glucose [6] and is regulated via Ca2+ signaling [7,8]. Metacyclogenesis from cultured epimastigotes [9] can be reproduced in vitro by using Triatomine Artificial Urine (TAU) medium [10] and Modified Insect Medium [11].
Another transformation step reproducible in vitro is amastigote formation (amastigogenesis) from tissue-culture trypomastigotes by treatment with the acidic medium [12]. This treatment mimics the biological conditions where intracellular trypomastigotes transform into amastigotes in the acidic phagolysosome [13]. Amastigogenesis is regulated by Ca2+ signaling [7] and is associated with the ubiquitin-proteasome pathway [14–16]. More recently, a method for amastigogenesis from metacyclic trypomastigotes has been reported [17].
Trypomastigote formation from amastigotes (trypomastigogenesis) is crucial for generating an infective form in the mammalian stage. Several lines of evidence suggest that trypomastigogenesis involves protein-specific degradation via the proteasome [14] and requires proline in the proline auxotrophic CHO-K1 cell line [18]. However, despite the pathogenic importance of this step, its reproduction in vitro has not yet been successful. In vitro induction of trypomastigogenesis would shed light on the molecular mechanisms of this process.
In the present study, we report a novel method for inducing in vitro trypomastigogenesis from the T. cruzi extracellular amastigote. Trypomastigogenesis can be induced using the metacyclogenesis medium—a simple combination of commonly used culture media: 80% RPMI-1640 and 20% Grace’s Insect Medium. Using this system, we show that trypomastigogenesis is regulated via inositol 1,4,5-trisphosphate receptor (IP3R)-mediated Ca2+ signaling. Our findings provide a new experimental tool for the physiological investigation of this parasite and throw light on the pathogenic importance of Ca2+ signaling in T. cruzi.
Methods
Trypanosoma cruzi culture
Epimastigotes of T. cruzi Tulahuen strain were cultured as previously described [19]. TcIP3R-SKO and EGFP-TcIP3R-overexpressing epimastigotes were cultured in liver infusion tryptose (LIT) medium (ATCC 1029) containing 0.25 mg/mL and 0.5 mg/mL G418, respectively [7]. Metacyclogenesis was performed as previously described [11]. Metacyclic trypomastigotes were added to the 3T3-Swiss Albino fibroblast cells (Health Science Research Bank, Tokyo, Japan), and the infected cells were passaged as described [20] until tissue culture trypomastigotes emerged in the culture supernatant. The tissue culture trypomastigotes were collected by centrifugation as described previously [20], and were thoroughly transformed into amastigotes by incubation with DMEM containing 0.4% BSA at pH 5.0 for 24 h, as described [12].
Induction of amastigote-to-trypomastigote transformation
The parasites in the culture supernatant were collected by centrifugation at 1,600 × g for 10 min. The resulting cell pellet was re-suspended in 80% (v/v) RPMI-1640, HEPES medium (Life Technologies, Grand Island, NY, No. 22400–089) and 20% (v/v) Grace’s Insect Medium (Life Technologies, No. 11605–094). For some experiments, the previous formulation was supplemented with fetal bovine serum (FBS). All medium formulations were antibiotic-free. Amastigotes (1 × 107) were incubated with 10 mL of the transformation medium in tightly capped 25-cm2 culture flasks at 26°C for predetermined periods. The number of amastigotes, intermediate forms, and trypomastigotes was determined by direct microscopic observation.
Indirect fluorescent antibody assay (IFA)
The anti-trans-sialidase monoclonal antibody (MAb 39) was provided by Dr. Sergio Schenkman (Universidade Federal de São Paulo, Brazil). IFA was performed as previously described [7].
Results and Discussion
Incubation of amastigotes in the metacyclogenesis medium results in the induction of trypomastigote transformation
Biologically, epimastigotes resemble amastigotes; both forms can replicate by binary fission and are able to transform into their respective infective forms: metacyclic trypomastigote and bloodstream trypomastigote. Therefore, we hypothesized that trypomastigogenesis may be triggered in vitro in a manner similar to metacyclogenesis [11,21]. Amastigote preparations used for the experiments were easily obtained by treating the tissue-culture trypomastigotes with acidic buffer at 37°C for 24 h (Fig 1A) [12].
Amastigotes (1 × 106 cells/mL) were cultured in 80% RPMI-1640 plus 20% Grace’s Insect Medium for 1 day (A) or 4 days (B). Representative microscopic images are shown by using an inverted light compound microscope (Olympus, IX71, Tokyo, Japan) with 60x objective. A video of the same field is available in S1 Movie.
We first tested whether the metacyclogenesis medium (80% RPMI-1640 plus 20% Grace’s Insect Medium) could induce trypomastigogenesis. As expected, incubation of extracellular amastigotes in the metacyclogenesis medium at a cell density of 1 × 106 cells/mL at 26°C for 4 days led to the generation of the flagellated form of the parasite (Fig 1B). The culture contained fully developed trypomastigotes and an intermediate form, the latter of which looked amastigote but had an obvious flagellum (shown as “Intermediate” in Fig 1B). In contrast, the resulting trypomastigotes were very motile and looked rather short and stumpy (shown as “Trypomastigote” in Fig 1B. See also S1 Movie). This morphology was frequently observed in tissue-culture trypomastigotes compared to metacyclic trypomastigotes. These results suggest that our method can successfully induce trypomastigogenesis in vitro for the first time.
Unexpectedly, although trypomastigogenesis occurrs in the host cells at 37°C, the incubation of amastigotes at 37°C did not effectively induce trypomastigogenesis. The reasons for this phenomenon are unknown. However, since trypomastigotes derived from in vitro trypomastigogenesis are biologically tissue-cultured trypomastigotes as described below, our findings may contribute to the understanding of the molecular mechanisms involved in trypomastigogenesis as well as the extension of a flagellum from an amastigote.
Grace’s Insect Medium is essential for trypomastigogenesis
We next investigated the optimal conditions for in vitro trypomastigogenesis (Fig 2). In the metacyclogenesis medium, amastigotes began to sprout flagella at day 4 post-incubation. The maximum efficiency of flagellation was about 20% (including an intermediate form, see also Fig 1) and obtained at day 6 (Fig 2A). Longer incubation periods (>7 days) led to the death of the parasites.
(A) Amastigotes (1 × 106 cells/mL) were cultured in Grace’s Insect Medium, RPMI-1640 medium, 80% RPMI-1640 plus 20% Grace’s insect medium, or 70% RPMI-1640 plus 20% Grace’s insect medium containing 10% FBS for 7 days. The histogram depicts the percentage of intermediate forms and trypomastigotes, which was calculated by daily counting of the different forms by using IX71 with 60 x objective. More than 100 parasites were randomly counted. (B) The percentage of trypomastigotes is shown in Fig 2A. Data shown are the mean ± S.D. of 3 independent experiments. *P < 0.05, **P < 0.01.
We further examined the effect of the composition of the incubation medium on trypomastigogenesis. To investigate whether the individual components of the metacyclogenesis medium could induce trypomastigogenesis, amastigotes were incubated in either Grace’s medium or RPMI-1640. Notably, Grace’s medium alone could induce a comparable level of trypomastigogenesis to that induced by the metacyclogenesis medium by day 6. At day 7, we observed more dead parasites in Grace’s medium and the transformation efficiency was significantly lower than in the metacyclogenesis medium. These data suggest that Grace’s medium contains the essential factor(s) for trypomastigogenesis but it does not support the longer period required for parasite survival. In contrast, RPMI-1640 did not support efficient transformation of amastigotes. Furthermore, we found that the addition of fetal calf serum (FCS) to the metacyclogenesis medium (70% RPMI-1640; 20% Grace’s medium; 10% FBS) significantly increased the level of trypomastigote formation at day 7 (P<0.05, Fig 2B). We designated this medium as “trypomastigogenesis medium” and used it for further experiments. On the other hand, it is striking at day 4 and day 6 that the trypomastigogenesis medium significantly inhibited the transformation of amastigotes compared to the metacyclogenesis medium (Fig 2A). Since the metacyclogenesis medium induced a comparable level of trypomastigogenesis to that induced by the trypomastigogenesis medium by day 6 (Fig 2B), FCS may inhibit flagella extension of amastigotes. However, for longer periods of cultivation, FCS may supply nutrients for the parasites in order to produce trypomastigotes effectively.
Trypomastigotes derived from in vitro trypomastigogenesis are biologically tissue-culture-derived trypomastigotes
We compared the properties of trypomastigotes derived from trypomastigogenesis to those of tissue-culture-derived trypomastigotes (Fig 3). Tissue-culture-derived trypomastigotes express strong trans-sialidase activity, but metacyclic trypomastigotes express very little trans-sialidase activity [22]. The protein structures of these trans-sialidases have similar N-terminal catalytic domains but their C-terminal regions are different; the former containing 12 amino acid repeats and the latter lacking this repeat sequence. These can be distinguished by monoclonal antibody 39 (Mab 39), which recognizes the C-terminal repeat region of trypomastigote-specific trans-sialidase [23]. An indirect fluorescent antibody assay (IFA) with the anti-trans-sialidase antibody (MAb 39) was performed against tissue-culture trypomastigotes (Fig 3Aa) and metacyclic trypomastigotes (Fig 3Ab). Expression of trans-sialidase containing C-terminal repeats was detected only in tissue-culture trypomastigotes. IFA with MAb 39 was then performed against the parasites derived from trypomastigogenesis. The trypomastigotes expressed trypomastigote-specific trans-sialidase (Fig 3Ad, T). The amastigotes in trypomastigogenesis medium also expressed trans-sialidase after 6 d of incubation (Fig 3Ad and A) but not before the induction of trypomastigogenesis (Fig 3Ac). The intracellularly dividing amastigotes were not found to react with Mab 39 according to previous reports [23], but trans-sialidase enzyme activity was detected in fully matured amastigotes just before trypomastigotes were observed in the host cell. The Mab 39-positive amastigotes observed in the trypomastigogenesis medium might be similar to these parasites.
(A) Tissue-culture trypomastigotes (a), metacyclic trypomastigotes (b), amastigotes (c), or the parasites cultured for 6 d in trypomastigogenesis medium (d) were fixed, incubated with anti-trans-sialidase antibody, and stained with Alexa Fluor 488-labelled (green) secondary antibody. The nuclei (n) and kinetoplast (k) (blue) were counter-stained using Hoechst 33342. (B) Trypomastigotes derived from trypomastigogenesis or tissue-culture trypomastigotes (2 × 105) were incubated with 2 × 104 3T3-Swiss albino cells for 12 h. For calculation of the infectivity, the number of intracellular parasites in a total of 200 cells was counted after Giemsa staining. Data shown are the mean ± S.D. of 3 independent experiments. Statistical analysis between the groups was performed using Student’s t-test.
Next, we investigated whether trypomastigotes derived from in vitro trypomastigogenesis actually infect mammalian host cells (Fig 3B). Trypomastigotes derived from trypomastigogenesis and tissue-culture trypomastigotes were incubated with 3T3-Swiss albino cells for 12 h, and the number of infected amastigotes was counted. The number of infected amastigotes was not significantly different between the two groups (P = 0.14). In these experiments, the culture medium was incubated for 30 min in tubes after trypomastigogenesis before being used to infect the host cells. Since amastigotes do not swim due to the lack of flagella, most amastigotes remained at the bottom of the tubes. We recovered the trypomastigotes from the supernatant and found that the number of contaminating amastigotes was very few (data not shown). Furthermore, extracellular amastigotes of type I T. cruzi (e.g. G strain) efficiently invade into non-professional phagocytes, but type II T. cruzi have a limited ability to invade this cell type [24]. Since our studies utilized the Tulahuen type II T. cruzi strain [25], the possibility of infection of the extracellular amastigotes into the host cells was negligible. Taken together, these results indicate that trypomastigotes derived from in vitro trypomastigogenesis are biologically tissue-culture-derived trypomastigotes.
TcIP3R regulates trypomastigogenesis
IP3R is an intracellular Ca2+ channel that releases Ca2+ upon various stimuli via activation by IP3. We previously reported that Ca2+ signaling via T. cruzi IP3R (TcIP3R) controls a variety of the parasitic biological processes, including metacyclogenesis and amastigogenesis [5]. That is, reduced and increased levels of TcIP3R expression promote metacyclogenesis and amastigogenesis, respectively. In the present study, we were interested to know whether TcIP3R-mediated Ca2+ signaling is associated with trypomastigogenesis in the present setup (Fig 3). For phenotypic analysis, we used TcIP3R-knockdown and TcIP3R-overexpressing T. cruzi. For the TcIP3R-knockdown construct, we had previously established TcIP3R-single knockout (SKO) parasites in which one of three TcIP3R gene loci was disrupted and the level of TcIP3R transcript was reduced to two-thirds of that in wild type (WT). For TcIP3R overexpression, we used T. cruzi expressing N-terminally EGFP-tagged-TcIP3R (EGFP-TcIP3R) [7].
We compared the efficiency of trypomastigogenesis between WT, SKO, and EGFP-TcIP3R cells at all days. We found a significantly larger population of flagellated parasites (intermediate + trypomastigotes) in the SKO parasites, whereas EGFP-TcIP3R parasites showed the lowest transformation levels of all three (Fig 4A). Similarly, the population of trypomastigotes was significantly higher in the SKO parasites and lower in those of EGFP-TcIP3R than that of WT (Fig 4B). These results suggest that TcIP3R-mediated Ca2+ signaling plays a pivotal role in trypomastigogenesis, metacyclogenesis, and amastigogenesis, and that the reduced levels of Ca2+ release via TcIP3R is likely to drive the transformation into the infective state in T. cruzi.
(A) Amastigotes of WT or TcIP3R-SKO- or EGFP-TcIP3R-overexpressing parasites were cultured in a medium composed of 70% RPMI-1640 and 20% Grace’s Insect Medium supplemented with 10% FCS for 7 days. The percentage of the intermediate forms plus trypomastigotes was calculated daily. (B) The percentage of trypomastigotes is shown in Fig 3A. Data shown are the mean ± S.D. of 3 independent experiments. *P < 0.05, **P < 0.01.
Besides trypanosomatids, Ca2+ signaling is essential for the survival of other parasitic protists. For example, Ca2+ regulates a variety of vital functions such as motility, cell invasion, protein secretion, and differentiation in apicomplexan parasites including Plasmodium, Toxoplasma and Cryptosporidium [26–34]. Thus, Ca2+ appears to be critical for the survival of a range of parasitic protists, and our data indicate that Ca2+ signaling influences multiple developmental stages of T. cruzi
In the present study, we developed a novel and simple method to induce trypomastigogenesis in vitro. Although our research has provided the framework for generating trypomastigotes in vitro, we were unable to fully reproduce the robustness of trypomastigogenesis that occurs in mammalian host cells. First, only 10–15% of extracellular amastigotes incubated in trypomastigogenesis medium for 7 days transformed into tissue-culture trypomastigotes (Fig 2). Considering that almost all amastigotes in mammalian cells typically transform into trypomastigotes in 24 h, the rate of transformation in vitro is very low. One possible explanation for this discrepancy is that the parasites become weak due to the in vitro incubation with acidic medium for long durations. Additionally, trypomastigogenesis in mammalian cells occurs at 37°C, but the in vitro transformation is induced at 26°C more effectively. These results indicate that other factor(s) are required to reproduce trypomastigogenesis in vitro to the level of that which occurs in mammalian cells. However, our method provides important insights into the molecular cues underlying trypomastigogenesis, a process of great pathogenic importance in mammalian hosts. Furthermore, our method provides targets for inhibitory compounds of trypomastigogenesis, which is a critical step for parasite survival. We also show that TcIP3R-mediated Ca2+ signaling plays a fundamental role in the multiple differentiation steps of T. cruzi. Further analysis is necessary to identify the stimulating molecules that promote IP3 synthesis, leading to Ca2+ signaling in the different developmental stages of the parasite.
Supporting Information
S1 Movie. Microscopic movie of amastigote-to-trypomastigote transformation.
Amastigotes (1 x 106 cells/mL) were cultured in 80% RPMI-1640 plus 20% Grace’s Insect Medium for 4 days. The field of the video is identical to that of Fig 1B. Note that the trypomastigote is very motile and have an obvious flagellum.
https://doi.org/10.1371/journal.pone.0135726.s001
(M4V)
Acknowledgments
We thank Sergio Schenkman (Universidade Federal de São Paulo, Brazil) for advice and for the generous gift of Mab 39.
Author Contributions
Conceived and designed the experiments: MH JM KM TN. Performed the experiments: MH JM. Analyzed the data: MH JM HU KM TN. Wrote the paper: MH HU TN.
References
- 1. Rassi A Jr, Rassi A, Marin-Neto JA (2010) Chagas disease. Lancet 375: 1388–1402. pmid:20399979
- 2. Wainszelbaum MJ, Belaunzaran ML, Lammel EM, Florin-Christensen M, Florin-Christensen J, Isola EL (2003) Free fatty acids induce cell differentiation to infective forms in Trypanosoma cruzi. Biochem J 375: 705–712. pmid:12887332
- 3. Rangel-Aldao R, Triana F, Comach G, Abate T, Fernandez V, McMahon-Pratt D (1988) Intracellular signaling transduction in the differentiation of Trypanosoma cruzi: role of cAMP. Arch Biol Med Exp (Santiago) 21: 403–408.
- 4. Rangel-Aldao R, Triana F, Fernandez V, Comach G, Abate T, Montoreano R (1988) Cyclic AMP as an inducer of the cell differentiation of Trypanosoma cruzi. Biochem Int 17: 337–344. pmid:2847739
- 5. Gonzales-Perdomo M, Romero P, Goldenberg S (1988) Cyclic AMP and adenylate cyclase activators stimulate Trypanosoma cruzi differentiation. Exp Parasitol 66: 205–212. pmid:2840306
- 6. Tyler KM, Engman DM (2000) Flagellar elongation induced by glucose limitation is preadaptive for Trypanosoma cruzi differentiation. Cell Motil Cytoskeleton 46: 269–278. pmid:10962481
- 7. Hashimoto M, Enomoto M, Morales J, Kurebayashi N, Sakurai T, Hashimoto T, et al. (2013) Inositol 1,4,5-trisphosphate receptor regulates replication, differentiation, infectivity and virulence of the parasitic protist Trypanosoma cruzi. Mol Microbiol 87: 1133–1150. pmid:23320762
- 8. Lammel EM, Barbieri MA, Wilkowsky SE, Bertini F, Isola EL (1996) Trypanosoma cruzi: involvement of intracellular calcium in multiplication and differentiation. Exp Parasitol 83: 240–249. pmid:8682192
- 9. Camargo EP (1964) Growth and differentiation in Trypanosoma cruzi. I. Origin of metacyclic trypanosomes in liquid media. Rev Inst Med Trop Sao Paulo 6: 93–100. pmid:14177814
- 10. Contreras VT, Salles JM, Thomas N, Morel CM, Goldenberg S (1985) In vitro differentiation of Trypanosoma cruzi under chemically defined conditions. Mol Biochem Parasitol 16: 315–327. pmid:3903496
- 11. Gluenz E, Taylor MC, Kelly JM (2007) The Trypanosoma cruzi metacyclic-specific protein Met-III associates with the nucleolus and contains independent amino and carboxyl terminal targeting elements. Int J Parasitol 37: 617–625. pmid:17239886
- 12. Tomlinson S, Vandekerckhove F, Frevert U, Nussenzweig V (1995) The induction of Trypanosoma cruzi trypomastigote to amastigote transformation by low pH. Parasitology 110 (Pt 5): 547–554. pmid:7541124
- 13. Burleigh BA, Woolsey AM (2002) Cell signalling and Trypanosoma cruzi invasion. Cell Microbiol 4: 701–711. pmid:12427093
- 14. González J, Ramalho-Pinto FJ, Frevert U, Ghiso J, Tomlinson S, Scharfstein J, et al. (1996) Proteasome activity is required for the stage-specific transformation of a protozoan parasite. J Exp Med 184: 1909–1918. pmid:8920878
- 15. de Diego JL, Katz JM, Marshall P, Gutiérrez B, Manning JE, Nussenzweig V, et al. (2001) The ubiquitin-proteasome pathway plays an essential role in proteolysis during Trypanosoma cruzi remodeling. Biochemistry 40: 1053–1062. pmid:11170428
- 16. Queiroz RM, Charneau S, Mandacaru SC, Schwämmle V, Lima BD, Roepstorff P et al. (2014) Quantitative proteomic and phosphoproteomic pnalysis of Trypanosoma cruzi amastigogenesis. Mol Cell Proteomics.
- 17. Contreras VT, Navarro MC, De Lima AR, Arteaga R, Duran F, Askue J, et al. (2002) Production of amastigotes from metacyclic trypomastigotes of Trypanosoma cruzi. Mem Inst Oswaldo Cruz 97: 1213–1220. pmid:12563492
- 18. Tonelli RR, Silber AM, Almeida-de-Faria M, Hirata IY, Colli W, Alves MJ (2004) L-proline is essential for the intracellular differentiation of Trypanosoma cruzi. Cell Microbiol 6: 733–741. pmid:15236640
- 19. Iizumi K, Mikami Y, Hashimoto M, Nara T, Hara Y, Aoki T (2006) Molecular cloning and characterization of ouabain-insensitive Na(+)-ATPase in the parasitic protist, Trypanosoma cruzi. Biochim Biophys Acta 1758: 738–746. pmid:16797482
- 20. Nakajima-Shimada J, Hirota Y, Aoki T (1996) Inhibition of Trypanosoma cruzi growth in mammalian cells by purine and pyrimidine analogs. Antimicrob Agents Chemother 40: 2455–2458. pmid:8913446
- 21. Sullivan JJ (1982) Metacyclogenesis of Trypanosoma cruzi in vitro: a simplified procedure. Trans R Soc Trop Med Hyg 76: 300–303. pmid:7051451
- 22. Rubin-de-Celis SS, Uemura H, Yoshida N, Schenkman S (2006) Expression of trypomastigote trans-sialidase in metacyclic forms of Trypanosoma cruzi increases parasite escape from its parasitophorous vacuole. Cell Microbiol 8: 1888–1898. pmid:16824037
- 23. Frevert U, Schenkman S, Nussenzweig V (1992) Stage-specific expression and intracellular shedding of the cell surface trans-sialidase of Trypanosoma cruzi. Infect Immun 60: 2349–2360. pmid:1375197
- 24. Fernandes MC, Flannery AR, Andrews N, Mortara RA (2013) Extracellular amastigotes of Trypanosoma cruzi are potent inducers of phagocytosis in mammalian cells. Cell Microbiol 15: 977–991. pmid:23241026
- 25. Adesse D, Iacobas DA, Iacobas S, Garzoni LR, Meirelles Mde N, Tanowiz HB, et al. (2010) Transcriptomic signatures of alterations in a myoblast cell line infected with four distinct strains of Trypanosoma cruzi. Am J Trop Med Hyg 82: 846–854. pmid:20439965
- 26. Nagamune K, Hicks LM, Fux B, Brossier F, Chini EN, Sibley LD (2008) Abscisic acid controls calcium-dependent egress and development in Toxoplasma gondii. Nature 451: 207–210. pmid:18185591
- 27. Siden-Kiamos I, Ecker A, Nybӓck S, Louis C, Sinden RE, Billker O (2006) Plasmodium berghei calcium-dependent protein kinase 3 is required for ookinete gliding motility and mosquito midgut invasion. Mol Microbiol 60: 1355–1363. pmid:16796674
- 28. Ishino T, Orito Y, Chinzei Y, Yuda M (2006) A calcium-dependent protein kinase regulates Plasmodium ookinete access to the midgut epithelial cell. Mol Microbiol 59: 1175–1184. pmid:16430692
- 29. Wetzel DM, Chen LA, Ruiz FA, Moreno SN, Sibley LD (2004) Calcium-mediated protein secretion potentiates motility in Toxoplasma gondii. J Cell Sci 117: 5739–5748. pmid:15507483
- 30. Billker O, Dechamps S, Tewari R, Wenig G, Franke-Fayard B, Brinkmann V (2004) Calcium and a calcium-dependent protein kinase regulate gamete formation and mosquito transmission in a malaria parasite. Cell 117: 503–514. pmid:15137943
- 31. Lovett JL, Sibley LD (2003) Intracellular calcium stores in Toxoplasma gondii govern invasion of host cells. J Cell Sci 116: 3009–3016. pmid:12783987
- 32. Enomoto M, Kawazu S, Kawai S, Furuyama W, Ikegami T, Watanebe J, et al. (2012) Blockage of spontaneous Ca2+ oscillation causes cell death in intraerythrocitic Plasmodium falciparum. PLoS One 7: e39499. pmid:22792177
- 33. Morlon-Guyot J, Berry L, Chen CT, Gubbels MJ, Lebrun M, Daher W (2014) The Toxoplasma gondii calcium-dependent protein kinase 7 is involved in early steps of parasite division and is crucial for parasite survival. Cell Microbiol 16: 95–114. pmid:24011186
- 34. Koyama FC, Chakrabarti D, Garcia CR (2009) Molecular machinery of signal transduction and cell cycle regulation in Plasmodium. Mol Biochem Parasitol 165: 1–7. pmid:19393157