Intracellular Localization and Trafficking of Serine Proteinase AhSub and Cysteine Proteinase AhCP of Acanthamoeba healyi
Nội Dung Chính
Abstract
Proteinases have been proposed to play important roles in pathogenesis and various biologic actions in Acanthamoeba. Although genetic characteristics of several proteases of Acanthamoeba have been reported, the intracellular localization and trafficking of these enzymes has yet to be studied. In the present study, we analyzed the intracellular localization and trafficking of two proteinases, AhSub and AhCP, of Acanthamoeba healyi by transient transfection. Full-length AhSub-enhanced green fluorescent protein (EGFP) fusion protein was found in intracellular vesicle-like structures of transfected amoebae. Time-lapse photographs confirmed the secretion of the fluorescent material of the vesicle toward the extracellular space. The mutated AhSub, of which the pre or prepro region was deleted, was found to localize diffusely throughout the cytoplasm of the amoeba rather than concentrated in the secretory vesicle. Transfection of the construct containing the pre region only showed the same localization and trafficking of the full-length AhSub. A cysteine proteinase AhCP-EGFP fusion protein showed similar localization in the vesicle-like structure in the amoeba. However, using Lyso Tracker analysis, these vesicular structures of AhCP were confirmed to be lysosomes rather than secretory vesicles. The AhCP construct with a deletion of the prepro region showed a dispersed distribution of fluorescence in the cytoplasm of the cells. These results indicated that AhSub and AhCP would play different roles in Acanthameoba biology and that the pre region of AhSub and pro region of AhCP are important for proper intracellular localization and trafficking of each proteinase.
The genus Acanthamoeba, one of the amphizoic amoebae with ubiquitous distribution in human environments, has been known to cause granulomatous amoebic encephalitis in immune-compromised hosts and sight-threatening amebic keratitis, especially in contact lens users (15).
Proteinases have been known to play important roles in the metabolism, development, or survival of protozoa (16). Considering the high phagocytic activity of Acanthamoeba as a free-living organism and tissue-invasive behavior as a parasite, proteases would be involved in various processes of Acanthamoeba, such as pathogenesis, nutrient obtainment, and host tissue destruction. To date, several reports on the serine, cysteine, and metalloproteinases of Acanthamoeba were published (9, 12, 18, 19). Serine proteinase purified from culture supernatant was reported to play roles in host tissue invasion because of its strong activity against a broad spectrum of extracellular matrix and serum proteins of humans (12). The gene of the purified serine proteinase was characterized and named AhSub based on high homology with bacterial subtilisins (3). Cathepsin L-like cysteine proteinase genes were cloned from Acanthamoeba healyi and Acanthamoeba culbertsoni (3, 29). However, the specific function of these cysteine proteinases in Acanthamoeba is still unclear. The intracellular localization and trafficking of the enzymes may suggest their possible role in Acanthamoeba.
The sequence data of the subtilisin (AhSub) and cysteine proteinase (AhCP) of A. healyi suggested that they would be produced as a prepro enzyme. Pre and pro domains of subtilisin and cysteine proteinases were reported to play roles in localization or trafficking of the enzymes in several protozoa and bacteria (14, 17, 24).
In this paper, we demonstrate the intracellular localization, trafficking, and secretion of a subtilisin-like serine proteinase, AhSub, and cysteine proteinase, AhCP, by transient transfection as an enhanced green fluorescent protein (EGFP) fusion protein in live cells and determine the important domain of the proteinase for the proper localization, trafficking, and secretion of the proteinase by deletion mutation analyses.
MATERIALS AND METHODS
Amoeba.
A. healyi OC-3A strain (ATCC 30866) isolated from the brain of a granulomatous amoebic encephalitis patient (20) was obtained from ATCC and cultured axenically at 25°C in Proteose peptone-yeast extract-glucose liquid medium, containing 20 g/liter Proteose peptone, 1 g/liter yeast extract, 0.1 M glucose, 4 mM MgSO4, 0.4 mM CaCl2, 3.4 mM sodium citrate, 0.05 mM Fe(NH4)2(SO4)2, and 2.5 mM (each) Na2HPO4 and KH2PO4. The final pH of the medium was adjusted to 6.5.
Expression vector construction.
The pUbg vector with the Acanthamoeba ubiquitin promoter and EGFP as a reporter gene (13) was used to construct the expression vectors for this study. AhSub is composed of prepeptide of 20 amino acid residues, propeptide of 96 residues, and mature protein of 293 residues (3). AhCP is composed of prepropeptide of 93 amino acid residues and mature protein of 237 amino acid residues (4). As shown in Fig. total of six different expression vectors of full-length AhSub and five deletion mutants of AhSub and a total of five different expression vectors of full-length AhCP and four deletion mutants of AhCP were designed for transient transfection. Primer sequences for PCR amplification for all constructs are shown in Table . Each PCR product of AhSub was ligated into the vector by the EcoRI and SpeI sites, and each PCR product of AhCP was ligated into the vector by the NcoI and SpeI sites with C-terminal EGFP. Two amino acids coding for the SpeI enzyme site, threonine and serine, were inserted between the AhSub/AhCP and EGFP. Plasmid DNAs of 12 different constructs were prepared using the Miniprep kit (iNtRON, Korea).
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TABLE 1.
ConstructPrimer sequenceapUbAhSub(f)gF: CCG
CCATGG
CCATGCGCGCCGTCACCCCTCR: CCG
ACTAGT
GGCGGTGGGGTACGAAGCAGCpUbAhSub(pre)gF: CCG
CCATGG
CCATGCGCGCCGTCACCCCTCR: ATA
ACTAGT
AGCGAGAGCGCTAGCGCAGAGpUbAhSub(pre-pro)gF: CCG
CCATGG
CCATGCGCGCCGTCACCCCTCR: CCG
ACTAGT
AGCAAGACCCTTGAAGAGGCGpUbAhSub(pro-m)gF: AAT
CCATGG
CCACGCACGACCCGCTCACGGR: CCG
ACTAGT
GGCGGTGGGGTACGAAGCAGCpUbAhSub(m)gF: AAT
CCATGG
ACTTCGACTACTCCAAGCACGR: CCG
ACTAGT
GGCGGTGGGGTACGAAGCAGCpUbAhSub(pro)gF: AAT
CCATGG
CCACGCACGACCCGCTCACGGR: CCG
ACTAGT
AGCAAGACCCTTGAAGAGGCGpUbAhCP(f)gF: ATT
GAATTC
ATGCGTGCCTACTTCGTGGGTR: TAT
ACTAGT
GCACCGGGCGGAGTAAAGCAGpUbAhCP(pre-pro)gF: ATT
GAATTC
ATGCGTGCCTACTTCGTGGGTR: ATA
ACTAGT
CTGCGCGCTGGAGATGGAGACpUbAhCP(pro)gF: ATT
GAATTC
ATGTCTCTTGCCCCTCTTCACAGGR: ATA
ACTAGT
CTGCGCGCTGGAGATGGAGACpUbAhCP(m)gF: ATT
GAATTC
ATGAACTGCCTGTCCCAGAGCGGCR: TAT
ACTAGT
GCACCGGGCGGAGTAAAGCAGpUbAhCP(pre)gF: ATT
GAATTC
ATGCGTGCCTACTTCGTGGGTR: ATA
ACTAGT
AGCGAGAGCGCTAGCGCAGAGOpen in a separate window
Transfection.
Trophozoites of A. healyi grown to mid-log phase in a 25°C incubator were washed twice with phosphate-buffered saline (PBS) and resuspended in Proteose peptone-yeast extract-glucose culture medium. Cells were cultured overnight at 25°C in a six-well culture plate with 4 × 105 cells per well in 3 ml of culture medium. Four micrograms of plasmid DNA in 100 μl of amoeba culture medium mixed with 20 μl of Superfect (QIAGEN) was incubated for 10 min at room temperature and then diluted with 600 μl of culture medium. Adherent amoebae in a six-well plastic culture plate were washed once with PBS at room temperature. After removal of most of the PBS, DNA-Superfect mixture was added dropwise onto the cells. Cells were incubated at 25°C for 3 h to allow uptake of DNA-Superfect complexes. Cells were washed once with PBS, resuspended in 3 ml fresh growth medium, and incubated at 25°C for 24 to 48 h. Expression of the EGFP fusion protein was checked by fluorescence microscopy.
Flow cytometry.
Forty hours after transfection, cells were washed twice and resuspended in 2 ml of PBS. The number of transfected cells and the fluorescence of expressed EGFP among 1 × 106 cells were measured with a FACScalibur (Becton-Dickinson) to determine the transfection efficiency.
Fluorescence microscopy.
Transfected cells expressing EGFP fusion protein were selected and allowed to adhere to a glass-bottom cell culture dish (BD Falcon). The cells were analyzed using an Olympus IX 70 fluorescent microscope with cooled charge-coupled device camera (Roper Scientific). Alternatively, transfected amoebae were flattened with an agar overlay to observe detailed intracellular structures (27). EGFP fluorescence was achieved with a 500- to 530-nm band-pass filter. Images and time-lapse photographs were captured and analyzed through the Metamorph imaging system (Universal Imaging Corp.).
Labeling of endocytic compartments with Lyso Tracker.
Transfected cells were grown on a cell culture dish, rinsed with 1× PBS, and stained with 1 nM Lyso Tracker Red DND-99 (Molecular Probes, Leiden, The Netherlands) in medium without serum for 30 min at room temperature. Thereafter, cells were washed with PBS, fixed with 70% ethanol in PBS for 2 min at room temperature, and flattened on an agar overlay.
DISCUSSION
In this study, we have demonstrated the intracellular localization, trafficking, and secretory processes of proteinases AhSub and AhCP of Acanthamoeba healyi by transient transfection. The amoeba expressing full-length AhSub-EGFP showed the fluorescent vesicle-like structures in the cytoplasm and secreted the fluorescent material outside the cell. In the case of the amoeba transfected with full-length AhCP-EGFP, the fluorescent vesicle-like structures were identified as lysosome by Lyso Tracker staining. Various deletion mutant analyses revealed that the pre domain of AhSub and the prepro domain of AhCP are essential for appropriate intracellular localization and trafficking of these proteinases.
Subtilisins are usually synthesized as prepro enzymes, which are later posttranslationally activated to the active enzymes by cleavage of the pre- and propeptides (11). The roles of pre- and propeptides of subtilisin trafficking in bacteria have been studied by biochemical and molecular biological investigations. The prepeptide functions as the signal sequence required for protein secretion across the cytoplasmic membrane, and the propeptide has been proposed to function as an intramolecular chaperone for production of active subtilisin (1, 7, 22, 26). The role of pre- or propeptide in the protozoan subtilases was analyzed in PfSUB-1 (21). However, subtilases of apicomplexan protozoa, including PfSUB-1 of Plasmodium falciparum, PbSUB2 of Plasmodium berghei, and TgSUB2 of Toxoplasma gondii, are transmembrane proteins rather than secretory proteins (17, 23). Therefore, the pre region of PfSUB-1 cleaved at the endoplasmic reticulum during secretory transport may not affect the localization of the proteinase at secretory organelles (21). In the case of AhSub, the pre region-EGFP fusion protein was localized in the secretory vesicles and secreted toward outside of the amoeba. This result indicates that the pre region of AhSub would be essential for proper intracellular trafficking and secretion of the proteinase. This role of the pre domain of AhSub is more similar to that of bacterial subtilisins than that of apicomplexan subtilisins. Furthermore, the sequence analysis of AhSub indicated that AhSub is more closely related to bacterial than apicomplexan subtilisins (3).
Proteinase has been hypothesized as a sorting receptor/chaperone within the secretory pathway (2). In several protease families, propeptides function as intramolecular chaperones that are essential for correct folding of the catalytic domain during secretory transport (6). The prosequence of subtilisins may be required for the association of the proenzyme with the cell before the release of the mature active enzyme into the medium and/or for guiding the protein to the appropriate folding for the active conformation (5). We found that the premature construct without propeptide failed to secrete the proteinase, substantiating the possible role of propeptide. Compared to the small sized prepeptide alone (259 amino acid residues including EGFP), this improper trafficking of the premature construct could have resulted from masking of prepeptide due to the improper folding of the mature domain (533 amino acid residues including EGFP). As reported for other proteinases, the propeptide of AhSub may act as a chaperonin for appropriate protein folding of AhSub (2). The role of propeptide in the AhSub trafficking would be the next step to understand the full process of intracellular trafficking of AhSub in the Acanthamoeba.
The vesicle-like structures of the full-length AhCP-EGFP fusion protein exhibited the same localization with lysosome in the transfected amoeba. This result could clarify the biological function of AhCP originally suggested by Hong et al. (4). They reported that AhCP in Acanthamoeba may play a role in digestion of phagocytosed material rather than pathogenesis because the Northern blot analysis revealed higher expression of AhCP in a soil isolate than in a clinical isolate (4). The majority of the cysteine proteinases of the C1 family are known to be lysosomal enzymes that function in intracellular protein degradation. AhCP showed perfect conservation of amino acid residues in the motif, like mammalian cathepsin L (4).
The amoebae expressing the prepro region of AhCP-EGFP showed localization similar to that of the full-length AhCP-EGFP fusion protein. However, the amoebae transfected with the mature region of AhCP-EGFP showed the dispersed fluorescence in the cytoplasm. In the case of amoebae expressing the pro region, some cells exhibited similar localization with the cells expressing the prepro region. However, some of these cells also demonstrated dispersed localization in the cytoplasm, similar to the amoebae expressing only the mature region. The classical trafficking mechanism of lysosomal enzymes in mammals involves mannose-6-phosphate receptors (8). However, alternative targeting mechanisms have also been described for Saccharomyces cerevisiae and Leishmania (10, 14). In the case of carboxypeptidase Y of S. cerevisiae, the involvement of sequences in the pro region was reported previously (24, 25). The Leishmania showed the lack of a role for N-glycosylation on targeting to the lysosome (14). The pro region (from amino acids 21 to 93) of AhCP containing the N-glycosylation site (from amino acids 67 to 70) may play some role in localization and trafficking. Further studies on the functional role and mechanism of the pre region and N-glycosylation site of the pro region are recommended.
Acknowledgments
We thank Joanna Alafag for assistance in editing the manuscript.
This work was supported by a Korea Research Foundation grant (KRF-2001-042-F00031).
