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Infection and Immunity, December 1998, p. 5906-5914, Vol. 66, No. 12
0019-9567/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.
School of Dentistry, University of Minnesota, Minneapolis, Minnesota
Received 26 May 1998/Returned for modification 25 August 1998/Accepted 11 September 1998
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ABSTRACT |
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Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References
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By mimicking hemostatic structural domains of collagen,
Streptococcus sanguis (aggregation-positive phenotype;
Agg+) induces platelets to aggregate in vitro. To test the
hypothesis that aggregation occurs in vivo, S. sanguis
(Agg+ or Agg
suspension) was infused
intravenously into rabbits. The extent of hemodynamic and
cardiopulmonary changes and the fate of circulating platelets were
Agg+ strain dose dependent. Within 45 to 50 s of the
start of infusion, 40 × 108 CFU of the
Agg+ strain caused increased blood pressure. Thirty seconds
after infusion, other changes occurred. Intermittent
electrocardiographic abnormalities (13 of 15 rabbits), ST-segment
depression (10 of 15 rabbits), and preventricular contractions (7 of 15 rabbits) manifested at 3 to 7 min, with frequencies dose dependent.
Respiratory rate and cardiac contractility increased during this phase.
Blood catecholamine concentration, thrombocytopenia, accumulation of 111Indium-labeled platelets in the lungs, and ventricular
axis deviation also showed dose dependency. Rabbits were unaffected by
inoculation of an Agg strain. Therefore, Agg+
S. sanguis induced platelet aggregation in vitro. Platelet
clots caused hemodynamic changes, acute pulmonary hypertension, and cardiac abnormalities, including ischemia.
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INTRODUCTION |
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Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References
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Bacteria are exogenous factors that may be viewed as thrombotic agonists when introduced into the circulation (37, 38, 53). Certain strains of Streptococcus sanguis, a microorganism most commonly found in human dental plaque, induce human platelets in plasma to aggregate in vitro (17, 23-25, 52). Platelet aggregation in vitro occurs after a lag time of 1.5 to 15 min depending on the platelet donor and the strain of S. sanguis (24, 25, 50). When induced by the strains we have studied, aggregation is dependent upon expression of the platelet-aggregation associated protein (PAAP) on the streptococcal cell surface (14, 16). This protein contains a collagen-like structural motif which is essentially indistinguishable from the known platelet-interactive domains on types I and III collagen (13, 15, 16). Collagen and S. sanguis induce in vitro platelet responses similarly (13).
Collagen also induces platelet aggregation in vivo. When collagen was infused into the circulation of rabbits, platelet clotting occurred causing coronary vasospasm, myocardial ischemia and sudden death (40). S. sanguis bacteremias frequently cause an often fatal, disseminated intravascular coagulation shock-like syndrome in immunocompromised patients (12, 43, 51, 54, 55). In the immunocompromised, S. sanguis apparently enters the circulation through ulcerated mucous membranes secondary to cytotoxic immunosuppressive therapy and associated neutropenia. S. sanguis bacteremias also occur through life in apparently healthy people (11). Consequently, people with prior heart valve disease are at risk for infective endocarditis associated most frequently with S. sanguis bacteremias (11). S. sanguis apparently causes thrombotic infection of damaged heart valves involving the accumulation of platelets and fibrin (2, 10, 26) and expression of tissue factor (3, 4, 7). Yet it is unclear whether S. sanguis induces platelet aggregation in vivo.
Given the ability to induce aggregation in vitro and perhaps cause
coagulation-associated diseases, we hypothesized that a platelet
aggregating strain of S. sanguis could induce platelet aggregation or clots in the circulation. To test this hypothesis, we
first identified strains of S. sanguis that differed in
their ability to induce rabbit platelets to aggregate in vitro
(26). After intravenous infusion of an in vitro
aggregation-inducing strain (Agg+), platelets were analyzed
for signs of aggregation in vivo. Platelet clots would be expected to
cause changes in hemodynamic and cardiopulmonary variables. Preliminary
findings about some variables in vivo suggested that these expectations
were reasonable (30, 31). Therefore, arterial blood
pressure, heart and breathing rates, blood catecholamines, and
electrocardiograms (ECGs) were monitored and analyzed with sufficient
numbers of rabbits to permit comprehensive analysis of the
dose-response relationships. To ensure that platelet aggregation caused
the hemodynamic and cardiopulmonary changes, parallel control studies
in rabbits were conducted with pyrogen-free saline and a strain of
S. sanguis which did not cause rabbit platelets to aggregate
in vitro (Agg).
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MATERIALS AND METHODS |
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Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References
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Experimental design.
To test our hypothesis, apparently
healthy New Zealand White rabbits were studied before and after t = 0, when viable streptococci (expressed in CFU) were infused for
1 min (Fig. 1). In each rabbit, a
baseline set of hemodynamic and cardiovascular variables was obtained
(t = 
10 to 0 min), including heart rate, blood
pressure, standard three leads of the ECG, respiratory rate, platelet
count, and blood catecholamine level. The blood pressure, heart rate, and ECG were then monitored continuously from t = 0 to 7 and
at 10, 20, and 30 min. Intermittently, blood was sampled (3 ml each sample) for platelet counts and catecholamine analysis at baseline, t = 7 to 8 (catecholamines only), and t = 30
min. At t = 10 min, 111Indium-labeled platelets
were infused into the venous circulation of some rabbits. At t
30 min, the rabbits were euthanized.
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Animal protocol. All protocols, including euthanization of rabbits, were consistent with the Guiding Principles in Care and Use of Animals of the American Physiological Society and approved by the University of Minnesota Animal Care and Use Committee. Before entering the experimental protocol, rabbits were conditioned by daily gentle handling for 2 to 3 weeks.
Rabbits (diet, Purina Rabbit Chow; age, 5 to 6 months; weight, 3.2 to 4.2 kg; gender, males and females) were anesthetized with intramuscular (i.m.) xylazine hydrochloride (Rompum, 5 to 10 mg/kg of body weight and ketamine, 30 to 40 mg/kg). Supplements of ketamine or nembutal were given to maintain anesthesia, and xylocaine was injected intradermally to prevent discomfort during surgical procedures. The femoral vein was cannulated for the infusion of streptococci, 111Indium-labeled donor platelets, and the euthanizing agent. Arterial blood pressure was recorded through the carotid artery cannula. Viable S. sanguis cells suspended in sterile, pyrogen-free saline, or pyrogen-free saline alone were infused. Rabbits were euthanized by lethal intravenous injection of nembutal, and the lungs were removed.Bacterial strains.
Two representative strains of S. sanguis from our culture collection were selected for study and
were described in earlier reports (25, 26). Strain 133-79 was originally isolated from blood culture of a confirmed case of
subacute bacterial endocarditis and was obtained from R. Facklam,
Centers for Disease Control and Prevention, Atlanta, Ga. This was a
biotype I strain according to the phenotyping scheme of R. R. Facklam as described previously (24, 25) and fails to bind
amylase (20). Strain L50 was a biotype I isolate from human
dental plaque provided by William F. Liljemark, School of Dentistry,
University of Minnesota, Minneapolis. The original isolates were
purified, aliquoted, and stored at 20°C in skim milk. Aliquots of
pure cultures were thawed only once and used to inoculate Todd-Hewitt
broth for the experiments on a given day. Subculturing was minimized by
preparation and storage of large numbers of aliquots at one time.
Periodically the platelet aggregation phenotype of stored aliquots was
confirmed by in vitro aggregometry experiments. Strain 133-79 (Agg+) induced aggregation of human plasma (PRP) within 3 to 15 min in the platelet aggregometer (24, 25, 50). Strain
L50 (Agg) elicited no measurable response of platelets by
in vitro aggregometry (24, 25).
1, reflecting viability and differences in counting
sensitivity and accuracy of the techniques. Given the limitations of
the techniques, both strains were infused as equivalent numbers of
streptococcal cells expressed as CFU.
Platelet aggregometry. Platelet aggregation in vitro models the annular vortex of flowing blood and physiological temperature by study in the aggregometer (24). Strains 133-79 and L50 were harvested, washed, sonicated briefly, and resuspended to 2 × 109 cells per ml as previously reported (24, 25). Platelet-rich plasma was isolated from the blood of donor rabbits as previously reported for human samples, adjusted to 4 × 108 per ml with rabbit platelet-poor plasma, warmed to 37°C, and challenged with an equal number of S. sanguis cells in the aggregometer.
Platelets: labeling and in vivo analysis. Blood (27 to 36 ml in acid citrate-dextrose) was obtained from donor rabbits (sedated with ketamine and Rompum or nembutal) by sterile cannulation of deep branch of the femoral artery. To prepare 111Indium-labeled platelets, platelet-rich plasma was isolated and washed platelets were prepared and then incubated with indium-111-oxine (Amersham, Arlington Heights, Ill.) as described previously (26). The total radioactivity infused, A (in counts/minute), was determined from aliquots of the injectate as described previously (26, 46). More than 95% of radioactivity in the blood was determined to be platelet associated. The lungs were harvested, and samples were placed in preweighed vials and reweighed. The uptake of radioactivity, Ai, in the organ samples was counted with a Packard Gamma Counter, and the fractional uptake per gram was calculated as FU/gram = [Ai/mass of organ]/A, as described previously (26, 46).
Heart rate, blood pressure, and ECG. Heart rate, blood pressure, and ECG were recorded on a two-channel strip chart recorder and on analogue tape. Data on tape was transferred directly to a computer for subsequent evaluation. To facilitate analysis, data was reviewed using an expanded scale and rerecorded on the strip-chart recorder. The first derivative of the blood pressure record was determined with custom software. Differences in ECG and electrical axis were determined from both the strip chart recording and the computer display at selected time periods. ECG abnormalities were identified and verified by comparison to reference tracings. The deviation in electrical axis was determined from the vector geometry of the QRS complexes from the standard limb leads.
dP/dt. A continuous computer-generated display of arterial pulses and associated first derivative time curves were used to assess changes in cardiac contractility. A custom computer program determined the maximum change in pressure with respect to time (dP/dt) of the arterial pulse. The change in maximum dP/dt was calculated at baseline and postbacteremia times. Following a perturbation by intravenous nembutal in preliminary experiments (data not shown), the percentage change in the maximum ventricular and carotid pulse dP/dt were found to be directly related. Consequently, change in left ventricular contractility was indexed by determination of the maximum dP/dt in the carotid arterial pulse as also validated by others (1, 33).
Respiratory rate. The respiratory rate was measured by two methods. The respiratory fluctuations on the blood pressure recording were noted and counted. A fiberoptic probe detected movements of the nose, which were recorded on a strip-chart recorder. The two rates generally coincided, but the fiberoptic recording was given preference.
Catecholamine determination. Catecholamine concentrations (norepinephrine and epinephrine combined) in arterial blood were determined in triplicate by radioenzymatic assay (CAT-A-KIT; Amersham International). Replicate determinations showed a coefficient of variation of up to 30%. Dose dependency was evaluated by the frequency of rabbits showing change between baseline and t = 7 to 8 min. The dose-response relationship in those rabbits with known change in [CAT] was determined as a function of the frequency of the change in dP/dt (Fisher exact test, two-tailed tests).
Platelet counts. Platelet counts were determined with a hemocytometer by standard methods. Blood was taken for platelet counts at baseline, t = 7 to 8 min and at t = 30 min. At least two samples were counted at each bleed.
Calculations, data analysis, and statistics. To estimate heart work, the average carotid blood pressure multiplied by the heart rate was calculated as described earlier (26). The heart rate-blood pressure product is proportional to the pressure-volume work of the left ventricle or an estimate of the hemodynamic status of the rabbit.
Differences between doses, and Agg+ and Agg
phenotypes and sham saline groups were ascertained. Percentage change
(magnitude) and frequency of change were calculated to facilitate
evaluation of dose dependency. The frequency of occurrence was
evaluated by linear regression analysis and Fisher exact test
(two-tailed), while percentage change (magnitude) was evaluated only by
linear regression analysis. Differences in magnitude between baseline and postbacteremia values were evaluated by the Student t test.
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RESULTS |
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Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References
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Platelet aggregation in vitro. In response to strain 133-79, the mean lag time to onset of rabbit platelet aggregation in vitro was 2.0 min (range, 1.8 to 2.5 min; n = 6 rabbits). Strain L50 failed to induce aggregation of platelets from any rabbit tested.
Hemodynamic consequences.
Infusion of doses ranging from
4 × 108 to 40 × 108 CFU of the
Agg+ strain altered blood pressure and heart rate primarily
during the first 7 min, which changed the index of cardiac work (Fig. 2A to C). Initial preliminary studies in
rabbits suggested that hemodynamic changes would occur as a function of
dose (30, 31). Compared to the Agg+ strain,
infusion of 40 × 108 CFU of the Agg
strain (or physiological saline vehicle) caused virtually no change in
any measured parameter and the blood pressure and heart rate remained
at baseline values (Fig. 2A and B). The comparatively low
Agg+ dose of 0.1 × 108 CFU was infused
into two rabbits. Hemodynamics did not change from baseline after
infusion. In contrast, three rabbits infused with 100 × 108 CFU of the Agg+ strain became hypotensive
within 40 s and the blood pressure approached zero within 7 min.
During the first 7 min after infusion of 4 or 9 × 108
CFU of the Agg+ strain, the blood pressure response was
hypertensive (Fig. 2A). The time of maximal increase in blood pressure
was inversely related to dose (r = 0.78; slope
different from 0, P < 0.001 by linear regression
analysis). Similarly the average maximal percentage increase in blood
pressure decreased with increasing doses of the Agg+ strain
(r = 0.52; slope different from 0, P = 0.004). After infusion of 40 × 108 CFU
(n = 15 rabbits), the blood pressure response was
predominantly diphasic, first hyper- and then suddenly hypotensive.
During the hypotensive phase, the heart rate was markedly elevated
(Fig. 2B).
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Cardiopulmonary consequences. Within 3 min of initiation of infusion (t = 3 min), rabbits showed electrocardiographic abnormalities that changed over time, often reverting to normal and then abnormal in a single beat. For example, one rabbit showed abnormal electrocardiographic ST-segment depression and alternating premature ventricular contractions (PVCs) in Lead I through t = 10 min (Fig. 3). At t = 20 and 30 min, the heart rate remained elevated and ST-segment depression persisted. In comparison to baseline, the peak systolic pressure is delayed relative to the QRS complex (excitation of the ventricles) and the dichrotic notch in the pressure recording disappears. When seen during the first 7 min postinfusion, ST-segment depression usually continued through t = 30 min (data not shown for all rabbits). The dose of Agg+ S. sanguis was directly related to the frequency of ECG abnormalities at t = 3 to 7 min, with the regression line significantly different from zero (P < 0.01) (Fig. 4A). After infusion of 40 × 108 CFU of the Agg+ strain, 13 of 15 rabbits showed ECG abnormalities (Table 1). The most frequent abnormalities were ST-segment depression observed in 10 of 15 rabbits and PVCs in 7 of 15. With this dose, changes in the ventricular electrical axis at t = 30 min were seen in 11 of 15 rabbits (six showed right axis deviation and five left axis deviation). During the 30-min postbacteremia period, rabbits often developed more than one type of abnormal ECG pattern.
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strain.
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Platelet fate.
If they formed in vivo, then platelet clots
should be observed in the lungs (Fig. 5A)
and the fate of circulating platelets should be reflected in
thrombocytopenia (Fig. 5B). Both of these measures of platelet clotting
in vivo were shown to occur as a function of infused dose of
Agg+ S. sanguis. Platelet clots in the lungs
occurred in response to all doses when analyzed at t = 30
min, but appeared to maximize upon infusion of 9 × 108 CFU (Fig. 5A). The FU of 111Indium-labeled
platelets/g was not significantly different at doses of 9 × 108 and 40 × 108 CFU. After infusion of
40 × 108 CFU of the Agg strain, the
FU/gram was 3 standard deviations lower than after infusion of 0.1 × 108 CFU of the Agg+ strain. Platelets
cleared from the circulation to the spleen, but the FU/gram of spleen
decreased as a function of dose of Agg+ S. sanguis (r = 0.82; slope different than 0, P = 0.003 by linear regression analysis) (data not
shown). The platelet count at t = 7 to 8 minutes was
generally unaffected by infusion of up to 4 × 108 CFU
of the Agg+ strain (thrombocytopenia in one of seven
rabbits) (Fig. 5B). The frequency of thrombocytopenia was 80% after
infusion of 9 × 108 CFU and 100% after 40 × 108 CFU (data not shown). The percentage decrease in
platelet counts was significantly related to dose of Agg+
S. sanguis (r = 0.83; slope different than
0, P < 0.001 by linear regression analysis). Since
Agg+ strain doses of 
4 × 108 CFU did
not cause detectable thrombocytopenia, platelet counts were not
completed for rabbits given the Agg strain.
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DISCUSSION |
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Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References
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The Agg+ strain of S. sanguis induces
platelet aggregation or clotting in vivo as predicted by the in vitro
data. Aggregation in vitro is all-or-none with a dose-dependent delay
(23). In vitro, rabbit platelets aggregate in response to
the Agg+ strain in about two minutes. The experiments in
vivo had been designed to record hemodynamic and cardiopulmonary
responses upon a 1-min infusion of S. sanguis. Direct
evidence for platelet aggregation or clotting in vivo include
thrombocytopenia and, when compared to the Agg strain,
accumulation of 111Indium-labeled platelets in the lungs
(Fig. 5), but not in the spleen. Platelets normally clear from the
circulation to the spleen, but the 111Indium-labeled
platelets used as tracers do not. The frequency and extent of
manifestations of platelet clotting in vivo increase directly with the
dose of inoculated Agg+ S. sanguis.
Changes in heart rate and blood pressure occur more rapidly than would
be predicted by the two minute lag time for in vitro platelet
aggregation. The blood pressure and heart rate change 10 to 15 s
before completing the 1-min infusion of doses of Agg+
S. sanguis 
9 × 108 CFU and reach maxima
shortly thereafter (Fig. 2). In vivo clots may incorporate red blood
cells to increase the rate of accumulating volume and mass when
compared to aggregation of only platelet-rich plasma. An early
dose-dependent increase in circulating catecholamines would also be
expected to potentiate clotting in response to S. sanguis.
In vitro, physiological concentrations of epinephrine potentiate human
platelet aggregation in response to S. sanguis (27,
37a). The rapid increase in circulating catecholamines may
originate from post-sympathetic discharge (19) or endogenous platelet stores (27, 56). Upon release from platelets,
thromboxane A2 and serotonin will also potentiate aggregation.
Therefore, the changing hemodynamics suggest that platelet clots form
earlier and are probably larger in vivo than would have been predicted by in vitro experiments.
Regulated by a negative feedback system, cardiac output is equal to the stroke volume times the heart rate and is dependent upon the blood pressure gradient divided by the total peripheral resistance of the vascular bed. A clot-inducing material like S. sanguis in the vascular bed alters the resistance to flow. In response to Agg+ S. sanguis, platelet clotting caused increased pulmonary vascular resistance. The reduced venous return promoted the hypotensive phase (Fig. 2A). Ventricular contractility (dP/dt) and heart rate (Fig. 2B) increased to regulate stroke volume and restore cardiac output.
Consistent with the accumulation of platelet clots in the lungs, tachypnea developed rapidly, maximizing within 90 seconds of infusion of 100 × 108 CFU of the Agg+ strain. In response to 40 × 108 CFU, tachypnea maximized at about 3.2 min. Platelet clot-associated occlusion persisted in some rabbits, causing pulmonary hypertension. Pulmonary hypertension resulted in right axis deviation of the heart as observed in 6 of 15 rabbits. Even the dose of 9 × 108 CFUs of the Agg+ strain caused tachypnea frequently, but with low severity (Fig. 4C). The magnitude of tachypnea in experimental animals is dependent upon the number of injected glass microspheres and independent of the anatomic region of the lungs to which the beads embolized (32, 34). The responses to experimental embolism appear to be determined primarily by the magnitude of the pulmonary obstruction (45). Hence, tachypnea is best explained by persistent dose-dependent platelet clots in the pulmonary circulation as shown by the association between accumulation of 111Indium-labeled platelets in the lungs with thrombocytopenia (Fig. 5A and B).
In our model, the pulmonary changes and accumulation of 111Indium-labeled platelets in the lungs may underestimate the extent of platelet clots formed or trapped in the pulmonary circulation. Ketamine used in our protocol has been shown to cause ex vivo pulmonary vasodilation in rabbits (39), which would antagonize the accumulation of platelet clots. Hence the potential for S. sanguis to induce in vivo platelet clotting may be even greater than suggested by our data.
An important consequence of S. sanguis-induced platelet
clotting is ST-segment depression, which indicates heart ischemia (9). Evidence of ST-segment depression first appeared during the hypotensive phase, occurred as early as three minutes after infusion, and generally persisted until term (Fig. 3). All rabbits with
40 × 108 CFU showed increased respiratory rate,
diphasic blood pressure and thrombocytopenia, but only 13 of 15 rabbits
showed abnormal ECGs and only 2 of 3 showed ST-segment depression. The
frequency of abnormal electrocardiographic responses may reflect
inter-rabbit variations in fibrinogen levels, plasminogen activator
activity, platelet reactivity, displacement or disaggregation of
platelet clots, or the anatomy and function of the coronary
circulation, which might provide restoration of blood flow by reflexive
vasodilation. Coronary vasospasm accompanied in vivo platelet clotting
in response to intravenous collagen (40). It is unclear if
coronary artery vasospasm was reflected in the response to the
Agg+ strain, but a spectrum of vasoactive mediators may be
released in response to S. sanguis-induced platelet
clotting. Based on the hemodynamic and cardiopulmonary changes,
platelet clotting occurred upon infusion of only the Agg+
and not the Agg strain of S. sanguis.
During the 30 min of our protocol, platelet clots appear to persist and may become thrombotic. Thrombi, however, require the generation of thrombin and fibrin. In humans, platelet clots can occur in the absence of initiation of coagulation and the production of fibrin (49). In our model, initiation of coagulation through tissue injury and the cytokine-mediated expression of tissue-factor is unlikely to occur in only 30 min (18, 41). Based on in vitro data, the platelet clots would be expected to contain activated platelets in proximity to the endothelium. Thromboxane A2 released from activated platelets, for example, can "activate" endothelium (48, 57). Coagulation can be initiated on the surface of activated endothelium and platelets, generating thrombin and fibrin (22). The contact factor (intrinsic) system of coagulation can be assembled and activated within minutes on endothelial cells (or platelets). Therefore, the platelet clots may become more thrombus-like over time.
Activation of coagulation would also rapidly generate vasoactive bradykinin and plasminogen activators (47). These products of coagulation may act synergistically with thromboxane A2 and serotonin from activated platelets, and the elevated circulating catecholamines seen after infusion of Agg+ S. sanguis, to promote an arteriolar pressor response. Clearly there are several available mechanisms to cause rapid vasoconstriction. In contrast, the norepinephrine pressor response was probably not inhibited by nitric oxide during the hypotensive phase of the diphasic blood pressure response caused by 40 × 108 CFU of Agg+ S. sanguis. Nitric oxide production requires several hours for cytokine-mediated gene expression in response to related streptococci or gram-negative lipopolysaccharides (42). S. sanguis caused changes far too rapidly to be explained based on events requiring the translation of genes and synthesis of new proteins. The rapid expression of a set of vasoconstrictors and platelet clotting appear to be sufficient to promote vascular occlusion and contribute to persistent ST-segment depression and heart ischemia in our model. Hence, S. sanguis-induced platelet aggregation in vivo may trigger several complimentary mechanisms to promote thrombosis rapidly in the apparent absence of endothelial or atherosclerotic disease. Thrombocytopenia in response to S. sanguis may suggest the occurrence of disseminated intravascular coagulation (DIC). DIC can occur with gram-negative or gram-positive sepsis (6, 41) and is marked by thrombocytopenia and the deposition of fibrin in the microvasculature. The gram-positive Staphylococcus aureus induces DIC through activation of the coagulation cascade in vivo (36) and correlates with the ability of the microbe to induce platelet aggregation ex vivo (35). In our experiments, fibrin deposition was unlikely to have occurred coincidentally with the sudden hemodynamic and cardiopulmonary changes, or the onset of platelet clotting. Hence, platelet clotting in response to S. sanguis appears to occur in the absence of DIC.
Agg+ S. sanguis bacteremias also cause the
formation of thrombotic platelet vegetations in the rabbit model of
endocarditis (26, 46). The Agg+ strain induced
the formation of significantly larger vegetations than the
Agg strain. One day after infusion of Agg+
S. sanguis, the vegetation was a dense mass of aggregated
platelets and fibrin, with few isolated and trapped bacterial cells
comprising less than 1/100th of the cross-sectional area
(29). The development of the vegetation could be inhibited
by infusion of specific anti-fibrin antibody (58) or
reversed by administration of tissue plasminogen activator
(46). Comprised of fibrin and aggregated platelets, the
vegetation formed in response to the Agg+ strain of
S. sanguis was a thrombus. Since aggregation of human and
rabbit platelets also occurs in vitro (24, 25, 50) and in
vivo, as shown in this study, there are now three lines of evidence
that Agg+ S. sanguis can be thrombogenic. That
S. sanguis experimental bacteremia can induce signs of
thrombosis and heart ischemia is also of interest because of the
possible epidemiological relationship between dental infections and
myocardial infarction (5, 8, 44). Individuals in several
different populations who have suffered recent myocardial infarction
show a greater prevalence of periodontitis, pulpal abscesses, and other
oral infections than control subjects. Similar findings have also been
reported for stroke as an outcome variable (21). The
underlying biological basis for these epidemiological findings is
unclear. S. sanguis comprises about 30% of the population of bacteria in the complex microbial community of the dental plaque biofilm. Fragments of this biofilm containing S. sanguis and
other potentially thrombogenic microorganisms such as
Porphyromonas gingivalis (28) are detected as
bacteremias often through life (11), although the character
and amount of the inoculum is unknown. Since the frequency and
magnitude of these bacteremias may increase with the occurrence of
chronic infections such as periodontitis, it is tempting to speculate
that S. sanguis bacteremias may cause similar hemodynamic
and cardiopulmonary changes in humans as shown in rabbits. While the
data showed that comparatively low doses of pure cultures of S. sanguis caused in vivo responses, environmental regulation in the
biofilm may result in expression of bacteria that are more or less
thrombogenic. Platelet clotting in vivo suggests a new and novel
paradigm of cardiac dysfunction caused by a nonpathogenic commensal
bacteria from the oral cavity.
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ACKNOWLEDGMENTS |
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We thank Dorothy Aeppli and James Hodges for excellent statistical assistance, Urve Daigle for computer-assisted graphics, and Angie Witt, Gordon MacFarlane, and Nick Armstrong for technical support.
This work was supported by NIH/NIDR R01DE05501, R03DE07303, P30DE09737, and K16DE00270.
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FOOTNOTES |
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* Corresponding author. Mailing address: University of Minnesota School of Dentistry, Department of Preventive Sciences, 17-164 Moos Tower, 515 Delaware St. SE, Minneapolis, MN 55455. Phone: (612) 625-8404. Fax: (612) 626-2651. E-mail: mcherzb{at}maroon.tc.umn.edu.
Editor: V. A. Fischetti
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REFERENCES |
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Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References
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