Figures
Abstract
Background
Human African Trypanosomiasis (HAT) also called sleeping sickness is an infectious disease in humans caused by an extracellular protozoan parasite. The disease, if left untreated, results in 100% mortality. Currently available drugs are full of severe drawbacks and fail to escape the fast development of trypanosoma resistance. Due to similarities in cell metabolism between cancerous tumors and trypanosoma cells, some of the current registered drugs against HAT have also been tested in cancer chemotherapy. Here we demonstrate for the first time that the simple ester, ethyl pyruvate, comprises such properties.
Results
The current study covers the efficacy and corresponding target evaluation of ethyl pyruvate on T. brucei cell lines using a combination of biochemical techniques including cell proliferation assays, enzyme kinetics, phasecontrast microscopic video imaging and ex vivo toxicity tests. We have shown that ethyl pyruvate effectively kills trypanosomes most probably by net ATP depletion through inhibition of pyruvate kinase (Ki = 3.0±0.29 mM). The potential of ethyl pyruvate as a trypanocidal compound is also strengthened by its fast acting property, killing cells within three hours post exposure. This has been demonstrated using video imaging of live cells as well as concentration and time dependency experiments. Most importantly, ethyl pyruvate produces minimal side effects in human red cells and is known to easily cross the blood-brain-barrier. This makes it a promising candidate for effective treatment of the two clinical stages of sleeping sickness. Trypanosome drug-resistance tests indicate irreversible cell death and a low incidence of resistance development under experimental conditions.
Conclusion
Our results present ethyl pyruvate as a safe and fast acting trypanocidal compound and show that it inhibits the enzyme pyruvate kinase. Competitive inhibition of this enzyme was found to cause ATP depletion and cell death. Due to its ability to easily cross the blood-brain-barrier, ethyl pyruvate could be considered as new candidate agent to treat the hemolymphatic as well as neurological stages of sleeping sickness.
Citation: Worku N, Stich A, Daugschies A, Wenzel I, Kurz R, Thieme R, et al. (2015) Ethyl Pyruvate Emerges as a Safe and Fast Acting Agent against Trypanosoma brucei by Targeting Pyruvate Kinase Activity. PLoS ONE 10(9): e0137353. https://doi.org/10.1371/journal.pone.0137353
Editor: Frank Voncken, University of Hull, UNITED KINGDOM
Received: June 4, 2015; Accepted: August 14, 2015; Published: September 4, 2015
Copyright: © 2015 Worku 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: NW has highly acknowledged the Deutscher Akademischer Austauschdienst (DAAD) for the support (Ref.No.: A/10/90327).
Competing interests: The authors have declared that no competing interests exist.
Introduction
Human African Trypanosomiasis (HAT) also called sleeping sickness is a re-emergent disease, but does not attract much attention, probably because its impact is regional.
The two subspecies of T. brucei known to cause HAT are T. brucei gambiense (T. b. gambiense) and T. brucei rhodesiense (T. b. rhodesiense). A third subspecies, T. brucei brucei (T. b. brucei), is only infectious to animals and is commonly used as an experimental model for the two other parasite species [1,2,3]. The T. b. gambiense brings the chronic form of HAT in West and Central Africa, representing more than 98% of all reported cases. T. b. rhodesiense results in the acute form of the disease in East and Southern Africa, representing 2% of all reported cases. Until now, it has been estimated that the actual number of cases is at least 20,000–30,000 the vast majority of which are not diagnosed or treated [4].
Currently available drugs suffer from contraindications; meanwhile, patient demands for hospitalization and treatment is high [5,6,7]. Identification of innovative drug targets that are safe, efficacious, cost effective and easy to administer is therefore a research priority.
A new treatment option, nifurtimox-eflornithine combination therapy (NECT), recently listed under the essential drugs of WHO to treat neglected tropical diseases, seems promising except that it still produces side-effects in 68% of patients [8,9].
Some trypanocidal drugs have been previously investigated for their anti-cancer activities [10]. The probable similarities among trypanosome and cancer cells are their fast proliferation characteristics and their robust glycolytic pathway [11,12]. However, the glycolytic chain in T. brucei has a number of peculiarities. Most of its glycolytic enzymes are localized within membrane bound organelles called glycosomes and pyruvate is released out of the cells as a final product of the glycolysis instead of lactate in mammalian cells. T. brucei bloodstream forms essentially depend on glycolysis as many enzymes of the tricarboxylic acid cycle and cytochromes are not expressed in the mitochondrion [13]. This shows the physiological essentiality of pyruvate export in T. brucei. A recent study has also confirmed the role of pyruvate transporter blockage as a promising target in trypanosomes [14]. Recently, the dicarbonyl compound, ethyl pyruvate, has been shown to combat glycolysis-driven tumor cells through inhibition of the activity of glyoxalases, which are involved in metabolism of methyglyoxal [15,16].
However, this mechanism may not be the same in T. brucei cells because of the absence of a functional glyoxalase I enzyme [17]. Besides the speculated mechanisms of action of ethyl pyruvate at the cellular level e.g. inhibition of the NF-kappaB pathway may not apply for T. brucei [18].
Surprisingly, in the present study we observed a strong anti-trypanosomal activity of ethyl pyruvate. Our current results indicate that this is most probably brought about by inhibition of an important regulatory enzyme within the glycolytic pathway, namely pyruvate kinase. Inhibition of this enzyme was found to cause a significant and fast depletion of ATP and consequently death of trypanosome cells. These results indicate that ethyl pyruvate might be a lead compound which warrants further structural optimization to become a promising candidate for the treatment of trypanosomiasis.
Results
Effect of ethyl pyruvate on T. brucei cells proliferation and their energy metabolism
We first analysed the effect of increasing concentrations (1–20 mM) of ethyl pyruvate and its reduced form, ethyl lactate, on proliferation of the T. brucei cells (strain TC-221). The samples without ethyl pyruvate were considered as blank controls. The result revealed that ethyl pyruvate effectively inhibits cell proliferation with an IC50 of 2.03 ±0.25 mM. The minimum ethyl pyruvate concentration that gives maximum inhibition was 5 mM (Fig 1A). Interestingly, ethyl lactate did not inhibit the cells (Fig 1B). This was surprising, because the difference between the two compounds is just the presence of two additional protons in ethyl lactate.
A cell proliferation/viability assay was conducted in 96-well cell culture plates containing 2x104 cells, medium and ethyl pyruvate in a volume of 200 μl. After 24 hrs of incubation the AlamarBlue cell proliferation reagent (20 μl) was added and the absorbance was read: (A) Ethyl pyruvate; (B) Ethyl lactate; (C) For the time-dependency test 2x105 cells/ml were cultured in 24-well plates in the presence of different concentrations of ethyl pyruvate at 0 mM (■), 1 mM (▲), 2.5 mM (x) and 5 mM (□). After certain time intervals aliquots were removed and the number of vital cells was counted. (D) For cell-recovery test 2x105 cells/ml were cultured in the presence of ethyl pyruvate at 0 mM (■), 1 mM (▲), 2.5 mM (▼), 5 mM (□) for 3 hrs in 24-well plates. Then, the medium was removed and the cells were replenished with fresh medium without the ethyl pyruvate and further cultured for 24 hrs. At the indicated time points aliquots were removed and vital cells were counted. Cells were cultured at 37°C containing 5% CO2 in a 100% humidified environment, * p<0.05.
Next we analysed the effect of ethyl pyruvate at different time points of incubation. The proliferation of trypanosomes was completely inhibited at 5 mM ethyl pyruvate after 3 hrs of incubation indicating that ethyl pyruvate kills trypanosomes within a short time of contact. At lower concentrations of ethyl pyruvate the inhibitory effect was reduced. No inhibition was observed at concentrations <1 mM ethyl pyruvate (Fig 1C).
To analyse whether ethyl pyruvate inhibits trypanosomes irreversibly, trypanosomes were incubated with variable concentrations of ethyl pyruvate for 3 hrs, then the medium was removed and the cells were finally replenished in fresh medium in the absence of ethyl pyruvate for 24 hrs (Fig 1D). Cells exposed to low concentration of the ethyl pyruvate (≤ 2.5 mM) preserved their vitality, continued to proliferate and were capable of recovering from the cytotoxic effect of ethyl pyruvate. However, at a concentration of ≥5 mM the cells were irreversibly damaged and completely lost their cellular integrity.
In vitro drug resistance
The rationale of this test was to analyse whether the trypanosomes become resistant to treatment by ethyl pyruvate. Therefore, T. brucei parasites were cultured in medium containing sub-lethal concentrations of ethyl pyruvate of 1 mM and 2 mM, respectively, for 30 days accompanied by changing of the medium every two days. Then, the cells were subjected to increasing concentrations of ethyl pyruvate (1 to 20 mM) and the proliferation capacity was determined. The results finally showed that the parasites failed to develop resistance against ethyl pyruvate during the selected period of exposure at least under in vitro conditions (Fig 2A). In addition to ethyl pyruvate and ethyl lactate, the sodium salt of pyruvate was also tested for its effect on T. brucei cells proliferation. The result showed no statistically significant inhibition at least in the range from 0 to 15 mM (Fig 2B).
(A) Cells were treated with sub-lethal concentration of ethyl pyruvate, 1 mM and 2 mM, respectively, for 30 days in separate cell culture flasks. The medium and the trypanocidal compound were changed every two days. The control cells were left in fresh medium without ethyl pyruvate. On day 31, 2x104 cells/100μl from each flask were suspended a 96-well plate. Each cell group was treated with ethyl pyruvate at increasing concentrations ranging from 1 to 20 mM. Absorbance was recorded at 48 hrs of incubation. (B) The impact of pyruvate (0–20 mM) on cell proliferation was analysed as described in Fig 1.
Comparative anti-proliferative effects of pentamidine and suramin
Currently, the registered first-stage sleeping sickness treatment drugs are pentamidine and suramin. Suramin is an analogue of Trypan Blue that has been used for treatment of sleeping sickness for many years [19]. Pentamidine belongs to the class of aromatic diamidines previously designed for prevention and treatment of pneumocystic pneumonia, leishmaniasis and first stage infection of T. gambiense [20]. It was our intent to compare the anti-trypanosomal activity of ethyl pyruvate with these standard drugs used in sleeping sickness treatment. As demonstrated in Fig 3A the proliferation of trypanosomes is inhibited by pentamidine at quite lower concentrations compared to ethyl pyruvate. Suramin demonstrated anti-proliferative effects in the range of 100 nM and 1 μM, however no complete inhibition even after 48 hrs of incubation at the maximum applied concentration of 3855 nM was achieved (Fig 3B). The time-dependency test revealed measurable effects of pentamidine only at 48 hrs of incubation (Fig 3C). The death rate of pentamdine treated T. brucei indicated that more than 80% of the cells could be killed after 24 hrs of incubation and complete inhibition of cell proliferation was obtained only at the highest concentration of 128 nM and after 48 hrs. The cell-recovery tests with pentamidine confirmed its cytostatic effect at 64 nM and full cytotoxicity (non-recovery) at concentrations ≥128 nM at long term incubation (Fig 3D). Compared to pentamidine, ethyl pyruvate, however, was a very fast acting and irreversible growth inhibitor.
Cell proliferation/viability was assayed as described in Fig 1 with the exception of the use of (A) pentamidine and (B) suramin at variable concentrations. (C) Time dependency of anti-proliferative effects of pentamidine at variable concentrations (12.8 to 128 nM) was performed analogously to the experiments shown in Fig 1. Control samples contained 100 μl of fresh medium instead of a trypanocidal compound. Pentamidine concentrations used were: 0 nM (■), 12.8 nM (▲), 51.2 nM (▼), 64 nM (♦) and 128 nM (●). (D) Recovery test of T. brucei cells exposed to pentamidine was done in 24-well in the presence of pentamidine (12.8 nM to 128 nM). Pentamidine concentrations used were: 0 nM (■), 12.8 nM (▲), 51.2 nM (▼), 64 nM (♦) and 128 nM (●).The results depict the mean of three independent measurements (n = 3), *p<0.05.
Effect of ethyl pyruvate at cellular ATP level
The sudden loss of viability of trypanosomes at short-time incubation with ethyl pyruvate prompted us to look at the energy budget of the cells assuming that ATP depletion may be a possible cause of its extreme cytotoxicity against T. brucei. Our results revealed that the cellular ATP level was significantly hampered. There was a clear concentration-dependent loss of cellular ATP in the presence of ethyl pyruvate (Fig 4). The result indirectly demonstrated that ethyl pyruvate might hamper the glycolytic pathway which is the sole energy-rich phosphate delivering pathway in trypanosomes.
Trypanomomes (3x105 cells/well) were cultured in 24-well plates in the absence (control) or presence of ethyl pyruvate (1 to 20 mM) and incubated for 3 hrs at 37°C in 5% CO2. After incubation, cells were centrifuged at 1500 rpm for 10 min and supernatant was removed. The cell sediment was re-suspended smoothly in 500 μl of fresh medium. From this suspension 50 μl (equivalent to 3x104 cells) was added into a 96-well black opaque-walled plate in duplicates and mixed with 50 μl of test reagent per well. Luminescence was read at 560 nm. The actual ATP level was calculated from the trend line formula of the standard curve (n = 3), *p<0.05.
Effect of ethyl pyruvate on the activity of glycolytic enzymes
The results shown above let us assume that ethyl pyruvate most probably interferes with the glycolytic pathway in trypanosomes. The enzymes critical for the survival of blood stream form trypanosomes that might directly affect the ATP production are hexokinase-1 (HK-1), phosphofructokinase (PFK) and pyruvate kinase (PK). Therefore, we analyzed the specific activity of these glycolytic enzymes in trypanosome extracts in the absence and presence of 10 mM ethyl pyruvate. This concentration was selected because of its maximum effects obtained in all tests so far. As demonstrated in Fig 5A and 5B, ethyl pyruvate was unable to inhibit the activity of HK-1 and PFK in cell extracts. In contrast to these enzymes the activity of the PK was significantly inhibited at a concentration of 10 mM ethyl pyruvate (Fig 5C).
Specific activity of glycolytic enzymes in T. brucei cell extracts in the absence and presence of 10 mM ethyl pyruvate. (A) hexokinase, (B) phosphofructokinase and (C) pyruvate kinase. All cell extracts were pre-treated with ethyl pyruvate for 30 min before activity testing. All experiments were performed in triplicates (n = 3), * p<0.05.
In order to exclude a possible influence of cellular metabolites of the extract on PK kinetics we used purified PK from rabbit muscle for detailed kinetic studies. Thus, we analyzed the substrate-enzyme activity relation in the absence and presence of variable concentrations of ethyl pyruvate and phosphoenolpyruvate (PEP), respectively. Fig 6 shows the Km (± SD) values for the control (without ethyl pyruvate), and at different ethyl pyruvate concentrations in dependence of the substrate concentration. From the obtained saturation curves the Ki value was calculated. Data analysis revealed a competitive inhibition of PK activity by ethyl pyruvate with a Ki = 3.0±0.29 mM.
Enzyme activity was measured by following the production of ATP from the substrates phosphoenolpyruvate (PEP) and ADP as described in Materials and Methods. Enzyme activity expressed as nmole ATP/μl/s (ordinate) was recorded in dependence of increasing substrate concentrations (PEP) in the absence and presence of ethyl pyruvate. Controls were (●) without ethyl pyruvate (Km = 0.22±0.02 mM); (○) 5 mM ethyl pyruvate (Km = 0.51±0.03mM); (◊) 10 mM ethyl pyruvate (Km = 1±0.08mM) and (∆) 15 mM ethyl pyruvate (Km = 1.4±0.08mM). The pure enzyme from rabbit muscle (200 U/mg) was used for the experimental setup to avoid contamination bias in our cell extract. The Km and Ki values were calculated by SIGMAPLOT (Systat Softwarwe Inc.).
Cytotoxicity of ethyl pyruvate to human red blood cells
To prove whether ethyl pyruvate displayed advantageous selectivity of action against protozoa cells we performed ex vivo experiments by co-incubation of human red blood cells with the trypanosomes and ethyl pyruvate for 3 hrs, followed by cell counting and analysis of the red blood cell hemolysis. As expected, at 5 mM ethyl pyruvate only a few motile cells were observed while no significant change was seen in the red blood cell count (Fig 7A). The latter finding was substantiated by a non-significant release of hemoglobin from the red blood cells that remarks the ethyl pyruvate´s safety at least toward human erythrocytes when compared with the OD of totally haemolysed blood cells of the same sample used as a positive control (Fig 7B).
(A) 6x105 red blood cells were mixed to 2x105 T. brucei cells in 5 ml fresh medium in a flask. Cells were first incubated at 37°C in 5% CO2 for 24 hrs. Out of this 1 ml-aliquots were distributed into 24-well plates and incubated with 100 μl of increasing concentrations of ethyl pyruvate (1–15 mM). Controls contained cells without ethyl pyruvate but 100 μl of fresh medium. The cells were then re-incubated for 3 hrs. Afterwards, the number of trypanosomes and human erythrocytes was counted using a haemocytometer. (B) Effect of ethyl pyruvate (10 mM) on red blood cell haemolysis was determined by measuring the optical density of the medium containing the T. brucei and red blood cells co-incubated for 3 hrs. Before measurement, the cells were spun down by centrifugation. Total haemolysis of an equivalent number of cells (labelled as ‘Control’) was achieved by sonication (70% power, 5x5 sec) using an ultrasonicater. Cells without ethyl pyruvate were used as negative controls (labelled as ‘Blank’).
Phase contrast microscope video imaging of ethyl pyruvate exposed T. brucei cells
To visualize the effectiveness and fast acting property of ethyl pyruvate we performed video-recording and phase contrast microscopy of the trypanosome.
The videos showed the features of morphological changes of trypanosoma cells throughout the 3 hrs incubation time. The cell motility status generally indicates how fast ethyl pyruvate acts in killing these cells. The fast acting property of ethyl pyruvate can easily be confirmed by the slow or static motion of the previously active motile cells. The cytotoxic effect of ethyl pyruvate started already after 1 hr of exposure and complete inhibition of cell motility finally leading to cell death was observed after 3 hrs when incubated with 5 mM of the compound. In contrast to ethyl pyruvate, no visible effect was displayed when using pentamidine at the highest toxic concentration of 128 nM within the same time range. The videos show the control cells without treatment (S1 Video), cells treated with 128 nM pentamidine (S2 Video) and cells treated with 5 mM ethyl pyruvate (S3 Video).
Discussion
Even though the trypanosome genome was sequenced many years ago, no new breakthroughs in the treatment of HAT have yet emerged [21], despite the fact that some promising compounds are now in the development pipeline [22,23]. Notably, drugs such as suramin and nifurtimox with anti-trypanosomal activity have been tested in cancer therapy, too [24,25,26].
A common feature between tumor cells and trypanosomes is the high consumption of glucose. To cover its high energy demand, the parasite uses the host’s glucose for ATP production [27,28]. Within the glycolytic chain phosphoenolpyruvate is finally converted to pyruvate and ATP by cytosolic pyruvate kinase. Pyruvate is then released from the cell because of the lack of a canonical L-lactate dehydrogenase.
Analogously, many tumor cells exhibit a high aerobic glycolysis combined with a restricted oxidation within the respiratory chain [29]. Instead of pyruvate as in trypanonomes, L-lactate is produced by tumor cells which provide a growth advantage because of the repression of the immune system and promotion of cell invasion [30].
Recently, we have shown that compounds containing a dicarbonyl structure such as ethyl pyruvate, curcumin and different polyphenols are capable to kill tumor cells by inhibition of glyoxalases [25,31]. These enzymes prevent glycolysis-driven cellular damage by converting the toxic methyl glyoxal to D-lactate [32].
These findings prompted us to study the effect of ethyl pyruvate on trypanosomes which, like most tumor cells, have a high glycolytic rate. However, we are aware that T. brucei lacks glyoxalase I and uses trypanothione instead of glutathione unlike in mammalian cells. Nevertheless, we surprisingly found that ethyl pyruvate effectively inhibited proliferation of the trypanosomes.
In search of another target within the glycolytic pathway we analysed key enzymes which are directly involved in the regulation of ATP production in T. brucei, e.g. HK-1, PFK and PK [33]. While PFK and HK were not inhibited significantly, competitive inhibition of PK (Ki = 3.0±0.29 mM) by ethyl pyruvate has been ascertained for the first time. PK activity is relatively abundant in the cytosol of T. brucei and is responsible for the net ATP production by the cell. While most cellular ATP is consumed by hexokinase and phosphofructokinase which are not under regulatory control, inhibition of PK would lead to a rapid loss of cellular ATP. Recently, it was found that loss of PK is lethal to glucose-adapted cells [34]. These data corroborate our results that PK is a new target of ethyl pyruvate. Detailed kinetic analysis revealed a competitive inhibition of PK by ethyl pyruvate. Surprisingly, neither the enzyme nor trypanosome cells could be inhibited by ethyl lactate. The absence of any anti-proliferative effect of this compound suggests that the reduced form is either not taken up by the cells or not converted to ethyl pyruvate because these cells are deprived of lactate dehydrogenase. Admittedly, performing kinetic analysis with mammalian PK and not with purified enzyme from trypanosomes is obviously a drawback of our study. However, trypanosome PK similar to mammalian PK responds to fructose 2,6-bisphosphate as an allosteric activator and require Mg2+ ions for full activity [35]. Furthermore, pphylogenetic and structural analysis clearly showed that the enzymes of trypanosomatids and yeast belong within the same grouping of species and demonstrate optimal similarity [36].
We found complete inhibition of trypanosomes at 5 mM ethyl pyruvate within 3 hrs (Fig 1). This effect was irreversible as no recovery of the cells was observed. Although the concentration of ethyl pyruvate (5 mM) is slightly above the Ki-value of PK (3.0±0.29 mM) for ethyl pyruvate, it in turn seemed to be sufficient to initiate a progressive loss of cellular ATP.
Until recently, the development of drug resistance in microbes and protozoa has been a big challenge in therapeutic medicine. Thus, the lack of drug resistance development we observed in our in vitro experiments at least over a time laps of 30 days is very encouraging. This could be due to the attack of more than one target in trypanosomes since it is known that ethyl pyruvate also inhibits glyoxalase II in mammalian as well as yeast cells [15]. This enzyme is present in T. brucei cells but with yet undefined functions [37]. In contrast to the natural evolutionary pressure in parasites, it is possible that only 30 days of in vitro exposure might be too short to draw determinative conclusions. However, we also expect that the laboratory adapted T. brucei cells are capable of proliferating faster and possibly acquiring drug resistance in a shorter period of exposure.
It has been discussed that monocarboxylates, which are structurally analogous to ethyl pyruvate, affects cell proliferation by blocking the pyruvate transporter. This transporter usually brings the toxic accumulation of the endogenous pyruvate leading to cell death by acidification [38,39,40]. We addressed this question, by exposing trypanosomes with sufficiently higher concentrations of pyruvate. This should stop the efflux of the endogenous pyruvate that might cause the proposed intracellular acidification. However, the impact of extracellular pyruvate on vitality of the T. brucei cells was negligible (Fig 2B). This may indirectly indicate the requirement of the dicarbonyl structural element in ethyl pyruvate and that pyruvate transporters blockage might still not be the mode of action of ethyl pyruvate in T. brucei cells [39].
The selective action of ethyl pyruvate was also confirmed by our ex vivo investigation showing that human red blood cells were not struck by the compound. This is quite surprising because red blood cells are known to rely on oxidation of glucose to lactate and possess a very active glyoxalase system [41]. In contrast to tumor cells, the lack of damage to red blood cells by the generated methylglyoxal might be due to the absence of mitochondria since methylglyoxal was shown to target mitochondria for induction of cell death and also because of their high level of glutathione [42].
Unlike in T. brucei the red blood cells are known to release lactate and the T. brucei pyruvate transporter permeases are not related to MCTs from mammals [43]. These might also be optional reasons why ethyl pyruvate is safe for red blood cells but not to T. brucei. It should also be considered, that red blood cells might contain a high amount of unspecific esterases which could degrade ethyl pyruvate easily.
Ethyl pyruvate is a comparatively safe and fast acting agent against T. brucei. However, a relatively high concentration is required to observe optimal inhibition. This might be considered as a constraint when compared with the currently registered drugs acting in nanomolar or micromolar concentrations (Figs 1 and 3). Therefore, for in vivo application ethyl pyruvate has to be administered in a concentrated solution by infusion in order to get an effective level of at least 5 millimolar in animals or humans. This route of application was already applied in a phase II clinical study by using 450 mg/kg/day given in five divided doses without side effects [44]. Another possibility of minimizing the required high dose of ethyl pyruvate is to chemically modify the chain length of the alcohol of the ester in order to increase permeability and inhibitory activity. A similar approach was recently demonstrated for optimizing inhibitors for trypanosome PFK and Leishmania PK [45].
Conclusion
Our in vitro experimental study presents ethyl pyruvate as a fast acting, effective and safe trypanocidal compound. Pyruvate kinase has been identified as the new target of ethyl pyruvate. Inhibition of this enzyme was found to cause ATP depletion and sudden cell death. However, further comprehensive studies are needed with respect to Ki reduction and toxicity evaluation as well as metabolism in infected animal models. Then, its predefined property to easily cross the blood-brain-barrier could predict its future applicability against both stages of trypanosomiasis [46].
Materials and Methods
Blood specimen
Heparinized human blood was obtained from male healthy volunteers in the age of 30 to 40 years. All participants provided their written informed consent to participate in this study. The local ethics committee of the Faculty of Medicine of the University of Leipzig, Germany, approved this study in accordance to the ICH-GCP guidelines (reference number: 057–2010–08032010).
In vitro cultures of Trypanosoma brucei cells
Laboratory adapted T. b. brucei cells (strain TC-221) were obtained from Prof. A. Stich, Würzburg, Germany [47]. The cells were cultured in complete Baltz medium which was composed of 82% Baltz basic solution, 0.8% ß-mercaptoethanol, 0.8% penicillin/streptomycin (10,000 U/ml), and 16.4% heat inactivated fetal calf serum (FCS). Cells were cultured using 50 ml sterile cell culture flasks (Greiner Bio-One, Frickenhausen, Germany) at 37°C and 5% CO2 in 100% humidified environment. The medium was changed every 2–3 days.
Cell proliferation/viability assay
The AlamarBlue cell proliferation assay (Thermo Fisher Scientific, USA) has been used to measure the metabolically active cells. The principle behind this assay relates to the fact that metabolically active cells create a reducing environment that promotes the conversion of resazurin (non-fluorescent) to resorufin (highly fluorescent). The absorbance was measured using an ELISA reader/96-well multiscanner (Tecan, Crailsheim, Germany) at ex550/em630 nm.
Concentration-response test
The concentration-response assay was performed in 96-well cell culture plates to which 100 μl of a cell suspension (2x104 cells), 100 μl of the trypanocidal compounds at increasing concentrations and 20 μl of AlamarBlue was added. Control wells contained 200 μl of equal number of cells in fresh medium without trypanocidal compounds. The change in absorbance was recorded after 24 hrs of incubation. The drugs or compounds used in different experimental settings were ethyl pyruvate and ethyl lactate, pentamidine-isothionate, suramin and pyruvate (Sigma-Aldrich, Munich, Germany).
Time-dependency test
The time-dependency test was done in 24-well plates containing 1 ml of cell suspension (2x105 cells/well) and 100 μl of ethyl pyruvate at variable concentrations (1 to 20 mM), or an equal volume of fresh medium (control). Cells were incubated for 24 hrs at 37°C in a humidified environment containing 5% CO2. For cell counting, a Neubauer haemocytometer (Marienfeld, Lauda-Königshofen, Germany) was used. The number of moving cells was recorded after 1 hr, 3 hrs, 6 hrs and 24 hrs of incubation, respectively. Tests were done in triplicates and the mean and standard deviation were calculated.
Cell-recovery test
The cell-recovery test was done using 1 ml of cells (2x105 cells/ml) seeded into a 24-well plate to which was added 100 μl of ethyl pyruvate (1 to 20 mM) or pentamidine (12.8 nM to 128 nM). A volume of 100 μl of fresh medium without trypanocidal compounds served as a control. Cells were exposed to ethyl pyruvate and pentamidine for 3 hrs and 48 hrs, respectively, aliquots were removed and centrifuged (1500 rpm, 10 min, 5°C). The supernatant was carefully removed and the precipitated cells were re-suspended with 1 ml fresh medium without trypanocidal compounds and cultured for another 48 hrs. Vital cells were counted at the beginning of the re-suspension and continued at 1 hr, 3 hrs, 6 hrs, 24 hrs and 48 hrs afterwards. The tests were done in triplicate.
In vitro drug-resistance test
Primarily, cells were treated with sub-lethal concentrations of ethyl pyruvate (1 and 2 mM) for 30 days in separate cell culture flasks. The medium and the trypanocidal compounds were changed every two days. The control cells were left in fresh medium without ethyl pyruvate. On day 31, 100 μl of 2x104 cells per well were seeded in a 96-well plate. Each cell group was treated with ethyl pyruvate at increasing concentrations ranging from 1 to 20 mM. Controls were incubated in fresh medium without ethyl pyruvate. To each well 20 μl of the AlamarBlue reagent and absorbance was recorded after 48 hrs of incubation.
Cell extracts preparation and protein concentration determination
Cells were harvested and the pellets were first re-suspended at 1:4 ratio in a lysis buffer containing 25 mM Tris, 2 mM PMSF, 10% Glycerol, 1% Tritonx100, 2 mM EDTA and freshly added 0.3% protease inhibitor cocktail at pH 8.0. The suspension was repeatedly vortexed every 1–2 min within 15 min duration. The cell sediment was always kept on ice. Then the mixture was centrifuged for 15 min at 13000 x g and 5°C. The supernatant was carefully pipetted into a new Eppendorf tube and the sediment was discarded. The protein content of samples was determined according to Bradford [48].
Determination of the ATP content
Cellular ATP content was determined by means of the CellTiter-Glo luminescent cell viability assay according to the manufacturer’s instructions (Promega, Madison, USA). Briefly, cells were cultured in 24-well plates (4x104 cells/well) in the absence or presence of ethyl pyruvate (1 to 20 mM) and incubated at 37°C and 5% CO2 for 3 hrs. Cells were then mixed with test reagents and luminescence was read. A standard curve was prepared from ATP (10 nM to 1 μM) in medium to determine the actual ATP level in cells.
Enzyme activity assays
Hexokinase.
Hexokinase (HK) (EC 2.7.1.1) activity was measured following up the reduction of NAD+ through a coupled reaction with glucose-6-phosphate dehydrogenase. The increase in absorbance was determined spectrophotometrically at 340 nm wavelength according to [49]. Briefly, 100 μl of the cell extract was added to 3 ml of 50 mM Tris-buffer containing 13.3 mM MgCl2, 0.67 M glucose, 16.5 mM ATP, 6.8 mM NAD, pH 8.0, and glucose-6-phosphate dehydrogenase. The measurements were done in the absence and presence of 10 mM ethyl pyruvate, respectively.
Phosphofruktokinase.
The activity of phosphofructokinase (PFK) (EC 2.7.1.11) in T. brucei was measured at 340 nm in a coupled assay with aldolase (EC 4.1.2.13), glycerol-3-phosphate dehydrogenase (EC 1.1.1.8) and triosephosphate isomerase (EC 5.3.1.1) according to [50]. Activity of phosphofructokinase was measured using 100 μl of T. brucei cell extract.
Pyruvate kinase.
To determine kinetics in pyruvate kinase (PK) (EC 2.7.1.40) activity we first applied the indirect coupled assay using lactate dehydrogenase (LDH) as helper enzyme [49,50]. However, ethyl pyruvate was found to act itself as a substrate of LDH resulting in a concentration-dependent concomitant increase in oxidation of NADH to NAD+. Hence the activity of PK was evaluated by measuring the ATP production using the CellTiter-Glo Luminescent assay following the manufacturer’s instructions (Promega, Madison, USA). To determine the inhibition of PK activity in the cell extracts the reaction was initiated by adding 10 μl of the crude cell extract (1.17 mg/ml protein) to 2 ml of a reaction mixture composed of 200 mM Tris/HCl buffer, 15 mM MgCl2, 2 mM ADP, 3 mM phosphoenolpyruvate and 10 mM ethyl pyruvate (pH 7.0). The PK activity was read against a standard curve of ATP and expressed as (nM ATP/μl/s).
The PK kinetics assay was performed by measuring the enzyme activity at increasing concentrations of phosphoenolpyruvate (0.1 to 3 mM) in the absence and presence of ethyl pyruvate (5, 10 and 15 mM). Purified PK-1 from rabbit muscle (stock of 200 U/mg) was used for the test. The activity measurements were performed for 10 min at 20°C. The ATP luminescence measurement was done in a 96-well white opaque plate (Greiner, Frickenhausen, Germany) at 250 milliseconds ATP luminescence integration time using the SoftMax Pro 5.3 software. Finally, the Vmax, Km and Ki values were calculated to characterize the inhibitory effect of ethyl pyruvate at the enzyme. The observed data in the presence and absence of ethyl pyruvate were fit simultaneously for a competitive enzyme inhibition model shown by the equation below. Nonlinear regression fitting was accomplished with use of SIGMAPLOT (Systat Software Inc.) applying a weighting function of 1/Y2. PK activity was expressed as (nM ATP/μl/s).
Effect of ethyl pyruvate on human red blood cells
Heparinized human blood (5 ml) was centrifuged at 2000 rpm for 15 min and supernatant was removed. The cells were washed three times with 20 mM sodium phosphate, 150 mM sodium chloride (PBS), pH 7.4. Human red blood cells (5x105) were mixed to 2x105 T. brucei cells in 5 ml fresh medium in a 25 cm2 culture flask. Cells were incubated at 37°C and 5% CO2 for 24 hrs. Aliquots (1 ml) were taken and distributed into 24-well plates and incubated with 100 μl medium containing increasing concentration of ethyl pyruvate (1 to 15 mM). Controls contained cells without ethyl pyruvate but 100 μl of fresh medium. The cells were then incubated for 3 hrs. Trypanosome cells and blood cells were counted and the release of haemoglobin in the supernatant after cell centrifugation was measured photometrically at 540 nm. As a positive control a cell suspension of red blood cells was haemolysed using ultra-sonication to obtain complete hemolysis of a similar blood specimen not containing ethyl pyruvate.
Phase contrast microscopy and video recording
Culture flasks containing 5 ml of cells (107 cells/ml) were exposed to a final concentration of 5 mM ethyl pyruvate and 128 nM pentamidine. A control flask contained equal number of cells in fresh medium without trypanocidal compounds. All the cells were incubated for 3 hrs. For video recording, 5 ml cell suspension (107 cells/ml) was poured into a Nunclon culture dish (Sigma-Aldrich, Taufkirchen, Germany) with a bottom partially replaced by a glass-slide to increase imaging quality. The dish was closed with a custom made lid equipped with a CO2 adapter to allow for 5% CO2 supply in air. Cells were observed for three hours on an inverted phase contrast microscope (DMIRB, Leica) endowed with a 20x Objective (0.4 NA) and a 1x C-mount. The microscope was enclosed by a self-made thermo-box kept at 37°C to provide usual cell culture conditions. Videos were recorded every hour for untreated and pentamidine treated cells. For those cells treated with 5 mM ethyl pyruvate video recording was done every 30 min. The recordings were taken using a Phytec FireWire-CAM-111H with a frame rate of 15 fps. Each video sequence lasts 2 min.
Supporting Information
S1 Video. Phase contrast microscope video of live actively moving T. brucei cells.
A control flask contained (107 cells/ml) in 5 ml fresh medium without drugs and assigned as a negative control. The cells were incubated for 3 hrs and videos were recorded every hour (For details regarding the method please see the Materials and Methods section). A free downloadable version of Freemake Video Converter.exe software was used to sequentially put the video files together in one video file (Link: http://youtu.be/KIK_zZnJrCM) (login ID: netsanetworku; password: netsanet32000).
https://doi.org/10.1371/journal.pone.0137353.s001
(DOCX)
S2 Video. Phase contrast microscope video of pentamidine treated T. brucei cells.
A test flask contained (107 cells/ml) in 5 ml fresh medium treated with 128 nM pentamidine and treated as shown in S1 Video. (Link: http://youtu.be/xj5kKmWpz6o) (login ID: netsanetworku; password: netsanet32000).
https://doi.org/10.1371/journal.pone.0137353.s002
(DOCX)
S3 Video. Phase contrast microscope video of ethyl pyruvate treated T. brucei cells.
A test flask contained (107 cells/ml) in 5 ml fresh medium treated with 5 mM ethyl pyruvate and treated as shown in S1 Video (Link: http://youtu.be/xp72G_wZ8EU) (login ID: netsanetworku; password: netsanet32000).
https://doi.org/10.1371/journal.pone.0137353.s003
(DOCX)
Acknowledgments
We thank Angelika Schäfer for the generous technical supports during the laboratory experiments in the institute of Biochemistry, Faculty of Medicine, University of Leipzig. We greatly acknowledge Professor Wolfgang Schellenberger from University of Leipzig for his kinetic data analysis. All members of our research group in the Institute of Biochemistry, Faculty of Medicine, University of Leipzig, are highly appreciated for the team work and unreserved support. We appreciate the support of Professor Mary T. White from Wright State University, USA, for proof reading the manuscript.
Author Contributions
Conceived and designed the experiments: NW GB. Performed the experiments: NW. Analyzed the data: NW IW RK RT SK. Contributed reagents/materials/analysis tools: AS AD GB. Wrote the paper: NW GB.
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