(Received for publication, September 20, 1996, and in revised form, February 10, 1997)
From the Divisions of Biochemistry,
§ Microbiology, and ¶ Pharmacokinetics and
Metabolism, Central Drug Research Institute, Lucknow
226 001, India
A stage-dependent increase in the level of putrescine, spermidine, and spermine during intraerythrocytic growth of Plasmodium knowlesi in rhesus monkey erythrocytes was observed. Further, intraerythrocytic P. knowlesi-induced putrescine influx was found in trophozoite stage-infected erythrocytes and process was time- and temperature-dependent and showed saturable kinetics. Characteristics of induced putrescine influx appears in infected erythrocytes to be close to the normal erythrocytes in terms of affinity of putrescine to the putrescine transporter (Km 34.6 ± 3.8 µM as normal erythrocytes and Km 37.2 ± 5.2 µM in infected erythrocytes). However, the difference involves the significant increase in the putrescine influx rate after infection (Vmax = 4.21 nmol/min/1010 normal erythrocytes, compared with 11.6 nmol/min/1010 infected erythrocytes). Energy dependence, involvement of -SH group, and noninterference by amino acid, spermidine, and spermine in the putrescine influx process clearly demonstrate the presence of a distinct transporter for putrescine in infected erythrocytes. A putrescine conjugate N1,N4-bis(7-chloroquinoline-4-yl)butane-1,4-diamine (BCBD) was synthesized, which inhibits the putrescine influx in the P. knowlesi infected erythrocytes (Ki of 43.2 µM) as well as in vitro growth of P. knowlesi (IC50 value, 7.64 ± 0.97 ng/ml BCBD, 10.8 ± 0.45 ng/ml chloroquine). Addition of exogenous polyamines failed to reverse the inhibitory effect of BCBD in vitro. Administration of BCBD (24 mg/kg body weight, intraperitoneal, twice a day for 4 days) cured the Swiss mice infected with multidrug-resistant infection of Plasmodium yoelii. Therefore, inhibition of putrescine transport in malaria-infected erythrocytes offers a lead in the search of a new class of chemotherapeutic molecules against malaria.
Malaria remains one of the most important parasitic disease in the tropical countries. The global expansion of the disease has been attributed mainly to the failure of vector control programs and spread of Plasmodium falciparum resistance to chloroquine and other known antimalarial drugs (1). For the development of new molecules effective against resistant strains, a new target for rational drug design is imperative (2).
The naturally occurring polyamines, spermidine, spermine, and their
precursor, putrescine, are important regulators of growth and
differentiation in a wide variety of cell types including protozoan
parasites (3). Inhibition of polyamine biosynthesis could be a suitable
target to control proliferative disorders and infectious diseases
(4-6). Parasites of genus Plasmodia, during its
intraerythrocytic schizogony (I-ES),1
undergoes a complex developmental cycle resulting in 8-32 merozoites from a single parasite. However, normal erythrocytes are devoid of
polyamine biosynthetic machinery, and only traces of spermidine and
spermine are detectable (7). Postinvasion, as P. falciparum rapidly multiply and grow, polyamines and their peak biosynthetic enzymes like ornithine decarboxylase (ODC) and S-adenosyl
methionine decarboxylase increases in parsitized erythrocytes (7, 8). These polyamines at certain stage of Plasodium cell cycle trigger the
replication of malarial DNA and stimulate synthesis of specific proteins (9). These observations were confirmed further by the presence
of polyamine dependent -like DNA polymerase that catalyzes synthesis
of malarial parasite DNA during I-ES (10). ODC, which catalyzes the
rate-limiting step in polyamine biosynthesis, is irreversibly inhibited
by
-difluoromethyl ornithine (DFMO), an ornithine analogue (11).
This compound inhibits the proliferation of various cell types
including parasitic protozoan (12). Addition of DFMO to P. falciparum culture prevented the accumulation of putrescine and
spermidine in parasitized erythrocytes, thus resulting in the arrest of
malarial parasite growth at trophozoite stage, i.e. prior to
initiation of DNA synthesis (7). On the basis of the above available
evidence, it appears that polyamine may also regulate the I-ES of
malarial parasite. However, DFMO failed to inhibit the erythrocytic
schizogony of malarial parasite in vivo (13). No possible
biochemical basis has yet been established for refractoriness of DFMO
against blood stage malarial parasite infection in vivo.
Our efforts to investigate the putrescine transport system in malarial parasite-infected erythrocytes are based on three specific reasons. First, an increasing body of evidence suggests that refractoriness of tumor cells and protozoan parasites to inhibitors of polyamine biosynthesis is due to influx of polyamines across the membrane, and this transport is also subjected to regulation by environmental and physiological stimuli (14-16). Changes in the influx or efflux of polyamines provides an additional mechanism to regulate the intracellular polyamine contents (17). Second, it has been well established that I-ES growth of malarial parasite results in numerous biochemical, structural, and functional changes in the host erythrocytes membrane (18, 19) and increased permeability to a wide variety of structurally unrelated solutes via transport pathways that are functionally distinct from those known to operate in normal erythrocytes (2, 20). These parasite-induced pathways facilitate both entry of metabolic and biosynthetic substrates into infected erythrocytes and rapid efflux of potentially harmful catabolites (21). Finally, exogenous addition of putrescine to DFMO-inhibited in vitro culture of P. falciparum resulted in the resumption of growth (7) and DNA synthesis (9). On the basis of the above mentioned facts, we envisaged that putrescine might be available from plasma by increasing its transport across the red cell membrane in the parasitized erythrocytes to overcome DFMO inhibition of ODC.
To prove the above mentioned hypothesis, the roles of specific polyamines were studied during intraerythrocytic development of Plasmodium knowlesi (a simian malarial parasite) in rhesus monkey and P. knowlesi-induced putrescine transport system in the parasitized erythrocytes was characterized. In recent years, emphasis is on altred membrane transport in malaria-infected erythrocytes as a potential pharmacological target for antimalarial drug development (20, 21). We have designed and synthesized a putrescine conjugate, N1,N4-bis(7-chloroquinoline-4-yl)butane-1,4-diamine (BCBD) on the basis of characteristics of induced putrescine transport system in parasitized erythrocytes and established a correlation between inhibition of putrescine influx and antimalarial activity. A summary of a part of this work has been published previously in abstract form (22).
Healthy rhesus monkeys of either sex
weighing 4-6 kg were procured from the primate house of our institute.
[14C]putrescine hydrochloride and
[8-3H]hypoxanthine were obtained from Amersham
International Plc. UK; -DFMO was synthesized at Marion Merrel Dow
Inc. (Cincinnati, OH) and obtained through Walter Reed Army Institute
of Research. All other chemicals and biochemicals were obtained from
Sigma.
The infection of P. knowlesi was maintained in rhesus monkeys by serial blood passage with 1 × 106 infected erythrocytes, and parasitemia was recorded through microscopic examination of Giemsa-stained thin blood smears.
Enrichment of Different Developmental Stages of P. knowlesi-infected ErythrocytesBlood from healthy and P. knowlesi-infected monkeys (at different developmental stages of the parasite, viz. ring, trophozoite, and schizont) were collected in prechilled acid citrate-dextrose solution. The blood was passed through CF-11 column, and thereafter, erythrocytes (both normal and infected) were washed with phosphate-buffered saline (0.85% NaCl, 10 mM phosphate buffer, pH 7.2) and suspended in the same medium. Different developmental stage-specific P. knowlesi-infected erythrocytes were enriched using Ficoll-Conray gradient as described earlier by Joshi et al. (18), and an enriched population of parasitized erythrocytes (ring-stage infected ~85-90% pure, trophozoite 85-88% pure, and schizonts stage 90-95% pure) were obtained.
Extraction and Analysis of PolyaminesThe normal and
infected erythrocytes were lyzed by three brief cycles of freezing and
thawing (at 70 and 37 °C) followed by sonication (Branson Sonifier
B-12, microtip 15 s, 3 times at 15 watt). 4 to 6 volumes of
perchloric acid (0.3 M) were added to sonicated medium and
thereafter centrifuged at 10,000 × g for 30 min at
4 °C. Polyamines were analyzed in the clear supernatant by
reverse-phase high pressure liquid chromatography after preparing their
benzoyl derivatives according to method of Verkoelen et al.
(23).
Freshly prepared normal and
trophozoite-infected erythrocytes were used for putrescine influx
as described previously (24) with few modifications, and optimal
conditions were standardized. In brief, erythrocyte (both normal
and infected) were washed four times with Hepes buffer saline (134 mM NaCl, 2.7 mM KCl, 1.5 mM KH2PO4, 8.1 mM
Na2PO4, and 25 mM Hepes, pH 7.4)
and resuspended in the same medium at 37 °C. Erythrocyte suspension
(450 µl of 2-5 × 108 erythrocytes/ml) in
combination with appropriate reagent solutions was taken in an
Eppendorf tube and kept at 4/37 °C for 10 min for temperature
equilibration. Influx of putrescine was initiated by adding varying
concentrations of putrescine pulsed with 0.5 µCi
[14C]putrescine and incubated further at 4/37 °C for
the specified time. The reaction was terminated by transferring three
aliquotes of 145 µl each of erythrocyte suspension to another
Eppendorf tube containing 800 µl of ice-cold isotonic Mops-buffered
MgCl2 solution (106 mM MgCl2, 15 mM Mops, pH 7.4) layered over 250 µl of dibutylpthalate.
Tubes were immediately centrifuged at 10,000 × g (15 s
at 4 °C), and supernatant along with dibutylpthalate layer were
aspirated out. Traces of the solution on the inner wall were removed by
cotton swab saturated with ethyl alcohol. The cell pellet was lyzed by
brief freezing and thawing (70 and 37 °C) and deproteinized by
addition of 0.5 ml of trichloroacetic acid (5% w/v) followed by
centrifugation at 10,000 × g (10 min at 4 °C). The
radioactivity in the supernatant was measured after transferring 400 µl of supernatant to the 10 ml of water-based scintillation fluid
(Aquasol) in LKB, 1209 Rack-beta liquid scintillation counter. For
parallel control samples, [14C]putrescine influx was
determined by substracting values obtained by carrying out incubations
in the presence of 1.2 mM putrescine (25).
To
a stirred putrescine-free base (0.088 g, 1 mmol), 4,7-dichloroquinoline
(0.396 g, 2 mmol) at room temperature was added. The reaction mixture
was held at 140-145 °C for 4 h and then allowed to attain room
temperature. The solid residue was washed with cold ether several times
to remove unreacted substrates. The solid residue, free from the
starting material, was triturated with 2 N HCl (5 ml)
solution, cooled in an ice bath, filtered, washed with water, and
air-dried. The product was finally washed with ether to give 0.262 g
(64%) of colorless BCBD, m.p. 340 °C (Fig. 1).
The data are as follows: yield 64%; m.p. 340 °C; IR max (KBr)
cm
1: 3450, 3240, 3080, 3040, 2970, 1610, 1580, 1560;
1NMR
(DMSOd6), 400 MHz: 1.88 (s, 4H), 3.30, 3.78 (m, 4H), 6.88 (d, 2H), 7.68 (d, J = 8 Hz, 2H),
7.92 (s, 2H), 8.48 (m, 2H), 8.65 (d, J = 8 Hz, 2H),
9.62 (br, 2H); m/z 411 (M+). Anal.
Calcd for (C22H20Cl2N4)
(Mr 411): C, 64.23; H, 4.87; N, 13.63. Found: C,
63.83; H, 4.79; N, 13.52.
The in vitro antimalarial activity of BCBD was evaluated using short term culture of P. knowlesi (quotidian periodicity in vitro as well as in vivo) (26). In brief, P. knowlesi-infected cells synchronized at predominantly ring stage were obtained from infected monkey and suspended in the culture medium (RPMI supplemented with 10% normal monkey serum) to get a final concentration of 6% hematocrit and 1.5% parasitaemia. Test compounds were dissolved in ethanol:water (1:1) solution and further diluted with culture medium. After initiation of the culture, test compounds and 3[H]hypoxanthine (2 µCi/well) were added to each well as the culture plate was kept at 37 °C in candle jar module. After incubation for 20-22 h, the culture was harvested on glass membrane filter using automatic cell harvester (PHDTM Cambridge, MA). Filters were transferred to Triton-based scintillation fluid (333 ml Triton X-100, 5.5 gm 2,5-diphenyloxazole, 0.1 gm 1,4-bis[2-(5-phenyloxazolyl)] benzene, and 100 ml of toluene), and radioactivity was counted in an LKB, 1209 Rack-beta liquid scintillation counter.
In Vivo Antimalarial ActivityThe multidrug-resistant Plasmodium yoelii nigeriensis strain maintained in Swiss mice was used to evaluate the in vivo antimalarial activity (27). Four-week-old Swiss albino mice of either sex weighing 20-22 gm were infected with P. yoelii (1 × 106 infected erythrocytes) intraperitoneally. The BCBD was given intraperitoneally in 0.2 ml of water:ethanol mixture twice daily from days 0 to 3. Degree of parasitemia was recorded from Giemsa-stained thin blood smears (28). The animals which did not develop patent infection till day 28 were recorded as cured. The LD50 of BCBD was determined in Swiss mice (29).
The results of the polyamine profile at different developmental stages of malarial parasite (P. knowlesi) during intraerythrocytic schizogony in its host monkey erythrocytes are presented in Table I. Only traces of spermidine and spermine were present in the normal erythrocytes, while putrescine was undetectable. After invasion of the parasite, ring stage-infected erythrocytes showed a significantly elevated level of spermidine (~7.0 fold) and spermine (~3-fold), and putrescine also appeared as a new molecule. At trophozoite stage-infected erythrocytes, significant increase was found in all the three polyamines though the pattern of increase was different (~3.5-fold for putrescine, ~2.7-fold for spermine, and ~2.11-fold for spermine) as compared with ring stage-infected erythrocytes. Similarly, schizont infected erythrocytes showed further increase in the polyamine levels though the pattern of increase was again different (~2.5-fold for spermidine, ~2.41-fold for putrescine, and ~1.21-fold for spermidine). These observations clearly demonstrate stage-specific increases in the polyamine levels during I-ES of P. knowlesi.
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In our previous studies, increased putrescine influx was observed in
P. knowlesi-infected erythrocytes as compared with normal erythrocytes (30). Fig. 2 showed that putrescine influx
was quite low at 4 °C in normal erythrocytes (0.5 nmol/1010 erythrocytes after 5 min of incubation) which did
not increase significantly even after 30 min of incubation. In
contrast, at 37 °C, putrescine influx increased linearly with time,
reaching up to 2.0 nmol/1010 erythrocytes after 20 min. In
infected erythrocytes, putrescine influx was still very low at 4 °C
(0.75 nmol/1010 erythrocytes after 20 min). However, at
37 °C, there was a steep linear increase in the putrescine influx,
which reached 31.6 nmol/1010 erythrocytes after 15 min,
i.e. more than 11-fold higher as compared with that observed
in normal erythrocytes.
The concentration-dependent influx of putrescine was
investigated in normal and infected erythrocytes after 2 min of
incubation at 37 °C (Fig. 3). Data obtained from
concentration-dependent putrescine influx curve were
computed in the Lineweaver-Burk plot using SigmaPlot 5.0, and
parameters obtained using axis to axis regression analyses were
Km 34.6 ± 3.8 µM and
Vmax = 4.21 nmol/min/1010
erythrocytes and Km = 37.2 ± 5.2 µM and Vmax = 11.6 nmol/min/1010 erythrocytes for normal erythrocytes and
infected erythrocytes, respectively.
Competition studies were carried out to demonstrate the specificity of
the parasite-induced putrescine transport system in infected
erythrocytes using structurally related molecules like amino acids and
other polyamines. Serine, leucine, lysine, and aspartic acid
representing different substrate or each amino acid transport system
(A, L, Ly+, B) failed to exert any effect on the rate of putrescine
influx in infected erythrocytes (Table II, part I). Spermidine/spermine
share the putrescine transport system partially while DFMO showed no
competition with the putrescine. MGBG significantly inhibited the
putrescine influx though, structurally, MGBG differs from putrescine.
Therefore, observations from these studies indicate that
parasite-induced putrescine transport system was highly specific for
putrescine. Further competition studies were carried out with the
SH
group interfering molecules and metabolic inhibitors to investigate the
possibility of carrier-mediated process of putrescine influx in the
infected erythrocytes.
SH group blocker agents,
p-chloromercuric benzoate (pCMB) and
N-ethylmaleimide (N-EM) inhibited the putrescine influx up
to 85 and 93%, respectively, as compared with control (Table
II). Involvement of
SH group in the putrescine influx
process was further confirmed when pCMB and/or N-EM coincubated in
presence of dithiothreitol restricted the effect of pCMB and/or N-EM in
the putrescine influx process. In the presence of potassium cyanide,
sodium arsenate, iodoacetic acid, and dinitrophenol in the incubation
medium, the process of putrescine influx was inhibited significantly
and maximum effect (82%) was observed with dinitrophenol.
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Putrescine influx inhibition by BCBD was carried out by
Michaelis-Menten approach. Data obtained from influx inhibition curve were computed in the Lineweaver-Burk plot using SigmaPlot 5.0, and
parameters obtained using axis to axis regression analysis were
Ki 43.2 µM with mixed competitive
inhibitory pattern (Fig. 4).
Effect of BCBD of in vitro growth of P. knowlesi
was carried out by means [3H]hypoxanthine incorporation,
and thereafter, concentration response data were fitted to generalized
sigmoid function using nonlinear regression (31). Chloroquine as a
reference gave IC50 of 10.3 ± 0.45 ng/ml (Fig.
5A), and BCBD yielded IC50 value
of 7.64 ± 0.97 ng/ml (Fig. 5B).
Effect of BCBD in combination with different polyamines during short
term culture of P. knowlesi were determined using
[3H]hypoxanthine incorporation assay (Fig.
6). Putrescine did not affect the
[3H]hypoxanthine incorporation, while spermidine
partially inhibited the process. Spermine inhibited
[3H]hypoxanthine incorporation by 67% compared with
corresponding control. Therefore, high concentration of spermine seems
to be toxic to the parasite. BCBD inhibited the nucleic acid synthesis up to 58% at 25 µM concentration. Coincubation of
putrescine or spermidine failed to reverse the effect of BCBD. However,
cytotoxic effect of spermine against P. knowlesi culture in
combination with BCBD produced an additive effect on nucleic acid
synthesis of the parasite.
The in vivo effect of BCBD against infections with multidrug-resistant (MDR) strain of P. yoelii nigeriensis in Swiss albino mice was studied at two dose levels (Group 1, vehicle control; Group 2, 12 mg/kg body wt, twice daily, 0-3 day; and Group 3, 24 mg/kg body wt, twice daily, 0-3 day) (Table III). The results on day 4 showed that no parasitemia appeared in any of the BCBD-treated groups; whereas in vehicle control, all mice developed patent infection and average parasitemia was 9.55 ± 3.68%. All group 2 mice were negative till day 7 but subsequently developed patent infection while group 3 mice did not develop any patent infection up to observed period of day 28. Therefore, 96 mg/kg total dose treatment (group 2) suppresses the development of the parasitemia in P. yoelii-infected mice, and mean survival time was increased while 192 mg/kg total dose treatment of BCBD was found curative. LD50 value of BCBD determined after intraperitoneal administration in Swiss mice was 430 mg/kg body wt (confidence limit 265-698 mg/kg body wt).
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Polyamines are known to play an important role in cell
proliferation. We have, therefore, investigated how each specific
polyamine is involved with stage-dependent growth and
multiplication of malarial parasite during intraerythrocytic schizogony
and the polyamine based regulatory mechanism of the intra-erythrocytic parasite proliferation. Analysis of elevated polyamine levels in terms
of spermidine/spermine (SPD/SPM) ratio, which is indicative of cell
proliferation (32), revealed that this ratio in normal erythrocytes was
2.24. However, after invasion of malarial parasite, increase in the
polyamine profile was observed, and this ratio reached to 4.76 in
ring-infected erythrocytes. A threshold level of SPD/SPM (6.17) was
attained in trophozoite-infected erythrocytes. It is not surprising
that it is maximal at trophozite stage because major molecular
synthesis occurs during this stage (33) and resembles the late G1 phase
in eukaryotic cell cycle. Though maximum level of polyamines were found
in schizont-infected erythrocytes, there was decrease in the SPD/SPM
(3.03) due to a specifically higher increase in spermine profile as
compared with spermidine. Studies carried out with malarial parasite
-DNA polymerase and polyamines showed that in vitro
addition of polyamines (1 mM putrescine, 1.5-2.0
mM spermidine, and 0.1-0.3 mM spermine) in the
presence of 2 mM MgCl2 increases the P. falciparum
-like DNA polymerase activity many-fold. But in
contrast to these observations, higher concentrations of spermine
(0.5-1.0 mM) inhibit the enzyme activity (more than 90%)
(10). Therefore, terminal lowering of SPD/SPM in schizont-infected
erythrocytes may lead to arrest of DNA synthesis at the end of the
P. knowlesi growth cycle and corresponds with the completion
of multiplication phase during I-ES of P. knowlesi. This is
further supported by our findings that at ring stage of the P. knowlesi culture, addition of spermine to the culture medium arrest the nucleic acid synthesis ([3H]hypoxanthine
incorporation assay) while the same concentrations of putrescine and
spermidine do not interfere with the process (Fig. 6). Therefore, it
can be concluded that during I-ES of malarial parasite, elevated
concentrations of spermidine and spermine act as positive and negative
regulator, respectively. Further, putrescine that acts as a precursor
for spermidine and spermine is not detected in normal erythrocytes
while it appears in ring-infected erythrocytes also as its biosynthetic
enzyme, i.e. ODC. Inhibition of ODC by DFMO arrest the
culture growth at the trophozoite stage (8). This indicates the
importance of putrescine for proliferation of the malarial parasite.
Characterization of malarial parasite-induced putrescine transport
system in trophozoite-infected erythrocytes explains the biochemical
mechanism by which addition of exogenous putrescine reverses the
-DFMO inhibition of P. falciparum (7-9) and in
vivo refractoriness of blood stage malarial parasite infection to
-DFMO (13). In recent years, considerable interest has been generated in elucidating the structure, mechanism, and regulation of
the polyamine transport system due to its major role in the homeostasis
of intraceullar pool (16, 17). No molecular characterization of
polyamine transport beyond influx kinetics and competition studies has
yet been reported, and the exact mechanism of transport as well as
variety of transport systems involved is still debated (34). We found
that enhancement in the rate of putrescine influx in infected
erythrocytes was due to a marked increase in the corresponding Vmax value rather than to a significant decrease
in the affinity constant. These results seems to indicate that
increased requirement of polyamines for rapid growth and multiplication
of intraerythrocytic malarial parasite give rise to a compensatory
mechanism producing a remarkable induction of putrescine transporter
synthesis. In most mammalian cell types examined for polyamine
transport, it has been shown that induced polyamine transport is marked
by increase in the influx rate without affecting the affinities of the
substrate to the transporter (35-38). Energy dependence, involvement
of
SH group, and noninterference by amino acid, spermidine, and
spermine in the putrescine influx process clearly demonstrate the
presence of a distinct transporter for putrescine in malarial
parasite-infected erythrocytes.
The presence of a malarial parasite-induced specific transport system for putrescine in the infected erythrocytes suggests that required putrescine for growth and multiplication of the parasite can be obtained from the external milieu, and failure of biosynthetic inhibitors in such organisms is not surprising. Therefore, blockage of polyamine transport or replacement of natural polyamines by their analogues may constitute an effective strategy for the development of chemotherapeutic molecules (39). For the development of new chemotherapeutic molecules, we have used three different approaches. First, diamine [H2N(CH2)xNH2] and structural homologs of spermidine [H2N(CH2)xNH(CH2)yNH2] antagonize putrescine and spermidine influx in mammalian cells, and available evidence suggests that a minimum of four methylene groups (x or x + y = 4) or their equivalent are necessary for efficient interaction with the polyamine transport system (40-43). Second, conjugates of transporter substrate and other drugs have been used as a means of enhancing the intracellular access of the conjugated drug. This approach has been applied to the polyamine transporter, polyamine-nitroimidazole conjugate, and polyamine-chlorambucil conjugate and has been shown to augment drug accumulation in Erlich-ascites tumors cells with a resulting enhancement of cytotoxicity (44, 45). Finally, we have found that chloroquine shares the parasite-induced putrescine transport system in P. knowlesi-infected erythrocytes (46). We have succeeded in designing and synthesizing BCBD using the combined knowledge of all the three approaches mentioned above.
Putrescine influx in P. knowlesi-infected erythrocytes
was inhibited by BCBD in a dose-dependent manner, and the
cytocidal concentration of growth of intraerythrocytic parasite
(IC50 value of 7.64 ± 0.94 ng/ml) was found to be
many-fold lower than other known polyamine analogues or biosynthetic
inhibitors (47-49). The novelty of this approach is that inhibitory
effect of BCBD on the parasite growth and multiplication in the culture
medium is cytocidal as addition of exogenous polyamines fails to
reverse the effect of BCBD. The lack of reversal would be expected if the BCBD blocks the intracellular binding of the polyamines or displaces intracellular polyamines from their binding sites (39, 50).
It is of interest to compare the antimalarial properties of
N,N-bis[3-[(phenylmethyl)
amino]propyl]-1,7-diaminoheptane (MDL 27695, Merrell Dow Research
Inst., OH), the most potent molecular of bis (benzyl) polyamine
analogues series designed to interfere with polyamine biosynthesis and
function with in vivo antimalarial activity of BCBD (48).
MDL 27695 cures the Plasmodium berghei infection in
vivo with a total dose of 150 mg in combination with DFMO (2%
solution in drinking water), though the parasite appears on day-4,
while BCBD cures the lethal multidrug-resistant strain of P. yoelii infection at the dose of 192 mg alone, and no patent infection appears in mice infected with the malarial parasite. Further
LD50 doses of BCBD for mice ranges ~430 mg/kg body wt; one can assume that therapeutic index in the P. yoelii
infected is higher than 10, revealing the high efficiency of BCBD
in vivo against the P. yoelii. The exact site of
interaction of BCBD with putrescine transporter/other vulnerable
biomolecules in the malarial parasite remains unknown. However, our
results support the initial premise that inhibition of putrescine
influx in malaria-infected erythrocytes by BCBD constitutes an
effective strategy in the search for a new class of molecules against
resistant strain of malarial parasite.
We are grateful to Dr. C. M. Gupta for helpful discussions during the course of this work.