Heme Polymerase Activity and the Stage Specificity of Antimalarial Action of Chloroquine

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Vol. 282, Issue 1, 108-112, 1997

Heme Polymerase Activity and the Stage Specificity of Antimalarial Action of Chloroquine

Augustine U. Orjih

MLS Department, Faculty of Allied Health Sciences, Kuwait University, Sulaibikhat 90805, Kuwait, Arabian Gulf

	Abstract

Top Abstract Introduction Materials & Methods Results Discussion References

Plasmodium falciparum lysate, prepared from 2.7 × 10⁷ ring-infected erythrocytes and incubated with hemoglobin in sodium acetateat pH 5, incorporated a mean of 1.6 nmol of ferriprotoporphyrinIX (FP) into hemozoin in 18 to 22 hr. A similar preparation oftrophozoite lysate incorporated a mean of 3.6 nmol of FP intohemozoin in 4 to 6 hr. These findings indicate differences betweenheme polymerase activity (hemozoin production) at the ring andtrophozoite stages of malaria parasites. Intracellular hemozoinproduction was 90% inhibited at the ring and trophozoite stagesby 0.5 and 7 nmol of chloroquine/10⁶ infected erythrocytes. respectively. The inhibition killed therings but not the trophozoites, suggesting that mature parasitesmay have a mechanism for protecting themselves against chloroquine-FPtoxicity.

	Introduction

Top Abstract Introduction Materials & Methods Results Discussion References

Shortly after the invasion of erythrocytes, the protozoan parasite Plasmodium enters its ring stage of development and beginsto ingest and digest hemoglobin as it grows to trophozoite andschizont stages (Olliaro and Goldberg, 1995). In the 48-hr asexuallife cycle of P. falciparum, these developmental stages coverthe first 20 to 24 hr, the next 12 to 18 hr and the remainingperiod, respectively (Yayon et al., 1983). The rate of hemoglobincatabolism is highest at the trophozoite stage (Orjih et al.,1994). Heme polymerase is located in the acidic food vacuole ofthe parasite and uses FP that has been released from hemoglobinas substrate for biosynthesis of hemozoin (Chou and Fitch, 1992;Slater and Cerami, 1992). In this process, FP is polymerized to $beta$ -hematin (the principal component of hemozoin) and stored inthe food vacuole (Fitch and Kanjananggulpan, 1987; Slater et al.,1991). Incorporation of FP into hemozoin is believed to be a protectivemeasure by the parasite against self-destruction. NonpolymerizedFP has been shown to be highly toxic, damaging proteases and cellmembranes (Chou and Fitch, 1980; Gluzman et al., 1994; Orjih etal., 1981; Vander Jagt et al., 1987). It also binds chloroquinewith high affinity, which may account for the selective accumulationof this drug in parasitized erythrocytes (Chou et al., 1980).Chloroquine promotes but can also delay FP toxicity (Orjih etal., 1981).

Consistent with a proposed mechanism of the antimalarial action of chloroquine (Orjih et al., 1981), various studies haveshown that the drug inhibits FP polymerization (Chou and Fitch,1992, Egan et al., 1994; Slater and Cerami, 1992). However, chloroquinekills P. falciparum, specifically at the ring stage of development(Orjih et al., 1994; Ter Kuile et al., 1993; Zang et al., 1986),although it has been shown in cell-free preparations that it inhibitsthe heme polymerase activity of trophozoites (Slater and Cerami,1992).

The present study presents a comparison of the heme polymerase activity in P. falciparum rings and trophozoites, measurementof chloroquine inhibition of this activity in parasitized erythrocytesand determination of the effect of the inhibition on the viabilityof the parasites. The findings of the study may provide plausibleexplanations for the stage specificity of the antimalarial actionof chloroquine.

	Materials and Methods

Top Abstract Introduction Materials & Methods Results Discussion References

Parasite cultures. RPMI 1640 medium was used for growing malaria parasites and washing them after concentration through saponin hemolysis (Orjih,1996). It was prepared and supplemented with 4-(2-hydroxyethyl)-1-piperazineethanesulfonicacid, sodium bicarbonate and 10% human serum (blood group O-positive)according to Jensen and Trager (1977). Each liter was supplementedwith 2 g of glucose, 50 mg of hypoxanthine and 19.2 mg of gentamicinsulfate (1.62 mg/ml concentration of doubly distilled water).The malaria parasite studied was the chloroquine-susceptible HB-3strain of P. falciparum. The parasites were grown in stored bloodgroup O-positive human erythrocytes by the conventional method,with incubation in a gas mixture containing 3% O₂, 3% CO ₂ and94% N₂.

Hemozoin synthesis in hemolysates. Infected erythrocytes concentrated through saponin hemolysis were used in preparing hemolysates at both ring and trophozoitestages of parasite development. After concentration, a suspensionof the ring-infected erythrocytes was prepared in culture medium,and 2-ml aliquots, each containing a total of 2.7 × 10⁷ parasitized erythrocytes, were prepared in sterilized high-speedOak Ridge centrifuge tubes. For hemozoin synthesis at the ringstage, the ring-infected erythrocytes were hemolyzed immediately,whereas for synthesis at the trophozoite stage, the aliquots ofconcentrated rings were incubated for 20 hr before they were hemolyzed.To prepare hemolysates, each aliquot was centrifuged for 30 minat 27,000 × g, and the supernatant was discarded. The pellet wasresuspended in 2 ml of modified Krebs-Ringer phosphate buffersolution, pH 7.4, containing 68 mM NaCl, 50 mM NaHPO₄, 4.8 mMKCl and 1.2 mM MgSO₄, and the pH was adjusted by adding HCl. Thesuspension was centrifuged for 30 min at 27, 000 × g, and thesupernatant was discarded. The pellet was vortexed vigorouslybefore being frozen for 10 min in liquid nitrogen. It was thenthawed at room temperature; 2 ml of a 500 mM sodium acetate buffersolution, pH 5, was added to the lysate, and the tube was vortexedvigorously and sonicated briefly. The tube was placed on a slowlyrotating mechanical mixer in a 37°C incubator. Hemolysates ofrings were incubated for 18 to 22 hr, and those of trophozoiteswere incubated for 4 to 6 hr. After incubation, each sample wascentrifuged for 30 min at 27,000 × g, and the supernatant wasdiscarded. The pellet was resuspended in 2.5 ml of sodium acetatebuffer and centrifuged, and the supernatant was discarded. Thiswashing procedure was repeated with 2.5 ml of modified Krebs-Ringerphosphate buffer solution.

To extract hemozoin, the crude pellet (largely a mixture of cell membranes and $beta$ -hematin) was suspended in 2 ml of 2.5% sodiumdodecyl sulfate buffered with 25 mM Tris to pH 7.8 and left overnight(16 hr) at room temperature. It was then centrifuged for 60 minat 27,000 × g, the supernatant was discarded and the pellet waswashed once with 2 ml of sodium dodecyl sulfate buffer solution.The hemozoin was then analyzed as described previously (Orjihand Fitch, 1993

Measurement of chloroquine accumulation. Infected erythrocytes, concentrated through saponin hemolysis, were used for measurement of chloroquine accumulation at thering and trophozoite stages of parasite development. Ring-labeled[¹⁴C]chloroquine (specific activity, 2.36 mCi/mmol; New England NuclearResearch Products, Boston, MA) was added to each culture, andthe mixture was incubated at 37°C for 60 min. In every case, theinfected erythrocytes were suspended in fresh culture medium immediatelybefore the addition of [¹⁴C]chloroquine to ensure that the pH was adequately maintained.At the end of incubation, the suspensions were centrifuged at27,000 × g at 4°C for 30 min, and the supernatant fluid was separatedfrom the pellet. Both supernatant fluid and pellet were assayedradiochemically for chloroquine with the use of Opti-Fluor-O scintillationcocktail (Packard Instruments, Meriden, CT).

Antimalarial action of hemozoin inhibition. Normal synchronized cultures containing a mean of 3.5% parasitemia (±1 S.E.M. of 4 experiments) were used to study the effectof chloroquine on hemozoin production and parasite viability.The cultures were exposed to various concentrations of chloroquineat the ring or trophozoite stage of parasite development and incubatedfor $>=$ 20 hr. Control cultures were not exposed to chloroquine.Hemozoin was extracted and measured according to the standardmethod (Orjih and Fitch, 1993).

The therapeutic effect of hemozoin inhibition by chloroquine on P. falciparum rings was evaluated morphologically by countingparasites that grew to schizont stage, whereas the effect on trophozoiteswas evaluated by counting new ring-infected erythrocytes thatappeared in the culture after trophozoites have been exposed tochloroquine for 20 hr.

	Results

Top Abstract Introduction Materials & Methods Results Discussion References

In this study, the parasitemia levels in unconcentrated cultures of P. falciparum rings were 2% to 8%, and after concentrationby saponin hemolysis, the levels were 90% to 99%. The concentrationprocedure was necessary for heme polymerase activity and chloroquineaccumulation experiments to avoid uninfected erythrocytes complicatingthe results.

Heme polymerase activity. The total quantities of hemozoin produced in ring and trophozoite lysates are shown in figure 1. Values represent mean ± S.E.M.of triplicate experiments. Before hemolysate preparation, thequantity of hemozoin was 2 ±0.2 nmol of FP in ring-infected erythrocytesand 13 ±1.5 nmol of FP in trophozoites; after incubation, thevalues increased to 3.6 ±0.1 and 16.4 ±1.6 nmol of FP, respectively.The difference between the mean quantities of FP incorporatedinto $beta$ -hematin in the two hemolysates is statistically significant(P < .03 by the paired t test).

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Fig. 1. Heme polymerase activity (incorporation of FP into hemozoin) in cell-free preparations. Hemolysates of normal and P. falciparumring-infected erythrocytes were incubated in sodium acetate atpH 5 for 18 to 22 hr, whereas those of trophozoites were incubatedat the same conditions for 4 to 6 hr. Each lysate was preparedfrom 2.7 × 10⁷ erythrocytes. The total amounts of hemozoin produced were calculatedin nM of FP, and mean ± S.E.M. values of three experiments areshown.

Chloroquine accumulation. The total number of infected erythrocytes used in the chloroquine accumulation study was ~2.6 × 10⁷ in both ring and trophozoite cultures. The experiments were donethree times. At a steady state of accumulation, after 1 hr ofincubation, extracellular (i.e., unbound) chloroquine concentrationsdecreased, depending on the parasite stage and initial drug concentrationadded to the medium (fig. 2). For example, when 53 nM chloroquinewas added to the medium, the concentration decreased by 28% inring cultures and 66% in trophozoite cultures; when 318 nM chloroquinewas added to the medium, the decrease was 6% in the ring and 70%in the trophozoite cultures.

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Fig. 2. Chloroquine accumulation by normal and P. falciparum-infected erythrocytes: steady state concentrations of unbound (extracellular)drug. Mean ± S.E.M. values of three experiments are shown. $open circle$ ,Trophozoite-infected erythrocytes; $black-triangle$ , ring-infected erythrocytes; $black-square$ , normal erythrocytes.

Generally, chloroquine accumulation by P. falciparum-infected erythrocyte was a saturable process, reaching a maximum at ~0.8nmol/10⁶ ring-infected erythrocytes and 7 nmol/10⁶ trophozoite-infected erythrocytes (fig. 3). In cultures containing106 nM of added chloroquine, ring-infected erythrocytes accumulated80% less than that accumulated by trophozoites, and this differencedid not change much when the added chloroquine was 318 nM. Asshown in figure 3, the difference between chloroquine accumulationby uninfected erythrocytes and ring-infected erythrocytes wasnot as noticeable as it was with trophozoites; nevertheless, itwas statistically significant (P = .0001 by the two-tailed pairedt test). The use of highly concentrated infected erythrocytesimproved the sensitivity of drug accumulation measurement.

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Fig. 3. Chloroquine accumulation by normal and P. falciparum-infected erythrocytes: steady state concentrations of bound (intracellular)drug. Mean ± S.E.M. values of three experiments are shown. $open circle$ ,Trophozoite-infected erythrocytes; $black-triangle$ , ring-infected erythrocytes; $black-square$ , normal erythrocytes.

Antimalarial action of hemozoin inhibition by chloroquine. Various studies by other investigators have shown that chloroquine inhibits $beta$ -hematin synthesis in cell-free preparations.However, to demonstrate the therapeutic significance of this inhibition,the study must be carried out with viable parasites (Asawamahasakdaet al., 1994; Orjih et al., 1994; Orjih and Fitch, 1993). Whenring-infected erythrocytes were incubated for 20 hr in 106 nMnonradioactive chloroquine, producing an intracellular drug concentrationof 0.5 nmol/10⁶ ring-infected erythrocytes, hemozoin synthesis was inhibitedby 90% (fig. 4), and parasite growth was arrested. After an additional20 hr of exposure, the drug was washed away, and the cells weremaintained for an additional 3 days in normal medium to see whetherthe parasites would recover. They did not, indicating that theparasites had died.

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Fig. 4. Intracellular concentrations of chloroquine and inhibition of hemozoin production in P. falciparum-infected erythrocytes.To obtain the intracellular drug concentrations indicated fromleft to right, ring-infected erythrocytes were exposed to 106and trophozoite-infected erythrocytes were exposed to 106, 212and 636 nM chloroquine, respectively. Hemozoin in drug-treatedcultures was subtracted from that in untreated controls, and theresults were expressed as percentage of the controls. Mean ± S.E.M.values of three experiments are shown.

Antimalarial action of hemozoin inhibition on trophozoites was evaluated somewhat differently from that on the ring stage.The question here was whether the trophozoites would completetheir life cycle and produce infective merozoites. For this purpose,parasite growth was synchronized at the ring stage, and the culturewas incubated for 20 hr to produce trophozoites. The mean parasitemiain the culture was 3.5%, leaving sufficient uninfected erythrocytesin the culture for invasion by newly released merozoites. Thetrophozoites were then incubated for 20 hr in culture medium containing106, 212, 318 or 636 nM nonradiolabeled chloroquine. The steadystate amounts of chloroquine accumulated by trophozoites fromthese drug concentrations (fig. 3) have been compared with theantimalarial action of chloroquine (table 1). It shows that inall the chloroquine concentrations tested, trophozoites were ableto complete their life cycle and infect new erythrocytes. Totalparasitemia was, however, highest in the culture without chloroquine,indicating that some of the parasites have been killed or inhibitedin growth by the drug. The lowest total parasitemia (20-40% ofthe control; data not shown) was observed in cultures that containedthe highest amount of chloroquine (636 nM in medium or 7 nmol/10⁶ trophozoites).

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TABLE 1
Viability of P. falciparum trophozoites exposed to chloroquine
Appearance of parasite rings in the culture after 20 hr of incubation indicates viability.

	Discussion

Top Abstract Introduction Materials & Methods Results Discussion References

In this study, some differences between heme polymerase activity in rings and trophozoites of P. falciparum have been detected.Although equal numbers (2.7 × 10⁷) of infected erythrocytes were used, mean hemozoin synthesisin ring hemolysate was only 50% of that in trophozoites. The initialquantity of hemozoin in the lysates was also lower in the ringsthan in the trophozoites, but Slater and Cerami (1992) have shownthat hemozoin by itself does not have heme polymerase activity.They showed that heme polymerase activity increased linearly withprotein concentration in parasite lysate. Obviously, hemoglobin-freeP. falciparum parasites are expected to contain less protein atthe ring than at the trophozoite stage, and this may account forthe differences in hemozoin synthesis observed in the presentstudy. However, Dorn et al. (1995) have shown that protein-freehemozoin can promote formation of additional hemozoin. In thepresent study, there was more preexisting hemozoin in the trophozoitelysates than in the ring lysates, and this may have contributedto the differences in the results.

The nature of heme polymerase is still unresolved. Sullivan et al. (1996a) reported that recombinant or native histidine-richproteins of P. falciparum promoted the formation of hemozoin incell-free preparations, but Bendrat et al. (1996) found that phospholipidscaused rapid FP polymerization. Future studies with histidine-richproteins and lipids from rings and trophozoites of malaria parasitesmay help clarify the role of these molecules in hemozoin synthesis.

To demonstrate the pharmacological importance of heme polymerase, Slater and Cerami (1992) added various antimalarial drugsto hemolysates of P. falciparum trophozoites and found that ~1mM chloroquine was necessary to cause ~90% inhibition of hemozoinproduction. This drug concentration is on the high side and carriesthe risk of not acting selectively. High concentrations of chloroquineinhibit other metabolic processes, such as DNA replication andprotein synthesis, and kill bacteria (Ciak and Hahn, 1966). Excesschloroquine may also delay, rather than promote, the toxicityof FP (Orjih et al. (1981), the effector molecule that is expectedto kill malaria parasites when hemozoin production is inhibited.

For the inhibition by chloroquine of heme polymerase activity to be biologically relevant, drug concentrations in the testsystem should be comparable to those that have been found to inhibitintracellular hemozoin production. In the present study, ~90%inhibition of hemozoin production was observed when intracellularchloroquine concentration was 0.5 nmol/10⁶ ring-infected erythrocytes or 7 nmol/10⁶ trophozoite-infected erythrocytes, suggesting that the mechanism,possibly heme polymerase activity, that is responsible for hemozoinformation is more sensitive to choroquine in rings than in trophozoites.Chloroquine accumulates selectively in the food vacuoles of malariaparasites, and Yayon et al. (1985) assumed that the amount accumulatedwas directly proportional to the volume of the food vacuole. However,it has recently been demonstrated that chloroquine accumulationin P. falciparum-infected erythrocytes is dependent on the rateof FP generation (i.e., hemoglobin catabolism) by the parasites(Orjih et al., 1994). The volume of a food vacuole increases withparasite maturation, reaching a maximum at late schizont stage(Langreth et al., 1978); in contrast, hemoglobin catabolism andchloroquine accumulation reach their peaks at the trophozoitestage and decrease dramatically thereafter (Orjih et al., 1994).It has been recently reported that quinoline drugs bind to hemozoin,possibly in complex with FP (Sullivan et al., 1996b); nevertheless,hemozoin by itself may not account for drug accumulation in parasitizederythrocytes. Schizonts contain more hemozoin than do trophozoites,whereas trophozoites accumulate more chloroquine than do schizonts(Orjih et al., 1994).

This study has also shown that the therapeutic effect of hemozoin inhibition is dependent on the developmental stage of P.falciparum, being more lethal to rings than to trophozoites. Althoughsome dead parasites were observed when hemozoin production introphozoites was inhibited by 90%, the surviving trophozoiteswere able to complete their life cycle and infect other erythrocytes.When a comparable level of inhibition of hemozoin production wasinduced at the ring stage, none of the parasites completed thelife cycle. How intracellular FP kills malaria parasites in thepresence of chloroquine has not yet been established, but it isbecoming evident that some metabolic processes taking place inthe food vacuole, as well as this organelle itself, are susceptible(Ginsburg, 1996; Olliaro and Goldberg, 1995). When added externally,FP and FP/chloroquine complex lyse cells (Chou and Fitch, 1980;Orjih, et al., 1981), and in cell-free preparations, they havebeen shown to inhibit proteases (Gluzman et al., 1994; VanderJagt et al., 1987).

The above observations suggest the following explanations for the stage-specificity of antimalarial action of chloroquine.Hemozoin formation, a requirement for continued utilization ofhemoglobin as nutrient source, is readily inhibited by chloroquineat the ring stage of intraerythrocytic malaria parasite development.The excessive accumulation of chloroquine in mature parasitesmay be in part due to diversion of drug/FP complexes into hemozoin(Sullivan et al., 1996b), away from the actual targets of antimalarialaction. Also, at later stages of parasite development, excessnutrients have accumulated in the host erythrocyte (Zarchin etal., 1986), and there are parasitophorous ducts through whichextracellular macromolecules may be imported (Pouvelle et al.,1991).

	Acknowledgments

This work was done in part in the laboratories of Prof. C. D. Fitch (St. Louis University School of Medicine, St. Louis, MO).

	Footnotes

Accepted for publication March 6, 1997.

Received for publication October 8, 1996.

Send reprint requests to: Dr. Augustine U. Orjih, Kuwait University, Faculty of Allied Health Sciences, MLS Department, P.O. Box 31740, Sulaibikhat 90805, Kuwait, Arabian Gulf.

	Abbreviation

FP, ferriprotoporphyrin IX.

	References

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