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1 Department of Human Biology and Nutritional Sciences, University of Guelph, Guelph, Ontario N1G 2W1; 2 Department of Medicine, McMaster University, Hamilton, Ontario, Canada L8N 3Z5; and 3 Department of Sports Science and Physical Education, University of Odense, DK-5230 Odense, Denmark
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ABSTRACT |
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Top
Abstract
Introduction
Methods
Results
Discussion
References
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This paper examines the time course of changes in plasma electrolyte and acid-base composition in response to NaHCO3 and KHCO3 ingestion. It was hypothesized that skeletal muscle is involved in the correction of the ensuing plasma disturbance by exchanging ions, gasses, and fluids between cells and extracellular fluids. Five male subjects, with catheters in a brachial artery and antecubital vein, ingested 3.57 mmol/kg body mass NaHCO3 or KHCO3. While seated, blood samples were taken 30 min before ingestion of the solution, at 10-min intervals during the 60-min ingestion period, and periodically for 210 min after ingestion was complete. Blood was analyzed for gases, hematocrit, plasma ions, and total protein. With NaHCO3, arterial plasma Na+ concentration ([Na+]) increased from 143 ± 1 to 147 ± 1 (SE) meq/l, H+ concentration ([H+]) decreased by 6 ± 1 neq/l, and PCO2 increased by 5 ± 1 mmHg. There was no detectable net Na+ uptake by tissues. An increased plasma strong ion difference ([SID]) accounted fully for the decrease in plasma [H+]. With KHCO3, K+ concentration increased from 4.25 ± 0.10 to 7.17 ± 0.13 meq/l, plasma volume decreased by 15.5 ± 2.3%, [H+] decreased by 4 ± 1 neq/l, and there was no change in PCO2. The decrease in [H+] in the KHCO3 trial primarily arose in response to the increased [SID]. Net K+ uptake by tissues accounted for 37 ± 5% of the ingested K+. In conclusion, ingestion of NaHCO3 and KHCO3 produced markedly different fluid and ionic disturbances and associated regulatory responses by skeletal muscle. Accordingly, the physicochemical origins of the acid-base disturbances also differed between treatments. The tissues did not play a role in regulating plasma [Na+] after ingestion of NaHCO3. In contrast, the net influx of K+ to tissues played an important role in removing K+ from the extracellular compartment after ingestion of KHCO3.
potassium bicarbonate; sodium bicarbonate; hyperkalemia; metabolic alkalosis; plasma volume; fluid balance; hydrogen ion; Stewart model of acid-base balance
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INTRODUCTION |
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Top
Abstract
Introduction
Methods
Results
Discussion
References
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SKELETAL MUSCLE, comprising ~45% of the body's
total mass, is capable of rapid gas, ion, and fluid exchange with the
extracellular fluids (ECFs). The blood acid-base disturbances and
exercise performance in response to
NaHCO3 ingestion have been studied
since the 1920s and have been summarized recently (20, 26). Previous
studies have also shown that the changes in plasma
H+ concentration
([H+]) and
HCO
3 concentration
([HCO3]) in response to
small amounts (1 mmol/kg body mass or less) of ingested
KHCO3 (37, 38) are similar to
those seen with NaHCO3 (20).
However, the processes involved in the acute, nonrenal regulation of
arterial plasma ion and acid-base balance in response to ingestion of
these solutions are not well understood (20). Increases in plasma
[H+] and
[HCO3] resulting from
NaHCO3 ingestion appear to be due
to an increase in plasma Na+
concentration ([Na+])
and a decrease in plasma Cl
concentration
([Cl]; see Ref.
20). Although acute effects of
KHCO3 ingestion have not been
extensively studied in humans (28, 37, 38), a generalized response may
be obtained from the data of van Buren and co-workers (37, 38).
KHCO3 ingestion (1.0 mmol/kg body
mass over a 2-h period) resulted in no change in plasma
[H+]; however, plasma
[HCO3] increased from 25 ± 1.2 to 28 ± 1.5 meq/l during the 1st h after ingestion and
was restored by the 2nd h after ingestion. Ingestion of 0.75 mmol/kg to
1 mmol/kg body mass KCl or 1.0 mmol/kg body mass
KHCO3, over a 2-h period,
increased plasma K+ concentration
([K+]) by >0.5 meq/l
and aldosterone concentration from 0.6 to 1 µmol/l in the 2nd h after
ingestion. Neither the KCl nor the
KHCO3 treatments affected plasma
[Cl]. Increases
in plasma [K+] in
these studies were remarkably low compared with estimated rates of
intestinal K+ absorption,
suggesting, to us, that substantial
K+ was extracted from the
circulation by the tissues.
The physicochemical origins of plasma fluid and ion disturbances to ingested Na+ and K+ are expected to be different due to differences in their distribution and handling (28). The cations Na+ and K+ are absorbed by different mechanisms within the small intestine and have a different distribution in the body (3, 17). The bulk of Na+ absorbed from the intestinal tract remains in the ECFs and, if not fully excreted, will result in an increased ECF volume (ECFV); on the other hand, K+ rapidly enters intracellular fluid compartments (30). Accordingly, the origins of the acid-base changes are also expected to differ between NaHCO3 and KHCO3 ingestion. The present paper uses the physicochemical approach detailed by Stewart (34, 35) to quantify the origins of acid-base disturbances with respect to the independent variables: strong ion difference ([SID]), the total concentration of weak acids and bases (ATot), and CO2 (23, 25).
Previous research has demonstrated that the arm, representing inactive tissues, is capable of modifying the composition of perfusing blood during and after high-intensity exercise (24). The rapidity of gas and ion exchange processes indicated a primary involvement of skeletal muscle in the acute regulation of plasma ion and acid-base status. In the present study, the involvement of skeletal muscle in the correction of acute disturbances in fluid and ion balance resulting from NaHCO3 and KHCO3 ingestion was assessed. The amount of KHCO3 administered was about threefold greater than that used in previous studies (37, 38) and identical to that shown to be of ergogenic benefit with NaHCO3 (20). We tested the hypothesis that skeletal muscle in particular, and tissues in general, modify the fluid, ion, and acid-base composition of the perfusing blood back toward "normal" after NaHCO3 and KHCO3 loading. It was also hypothesized that skeletal muscle would play a greater role in regulating the disturbance resulting from KHCO3 loading than NaHCO3 loading, due to the 100-fold greater permeability of cell membranes to K+ compared with Na+.
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METHODS |
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Top
Abstract
Introduction
Methods
Results
Discussion
References
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Six healthy male subjects, age 27 ± 2 yr old and mass 78 ± 6 kg, participated. The order of presenting the experimental treatments was randomized and separated by at least 2 wk to allow for normalization of hematocrit (Hct). Written informed consent was obtained after the procedures and potential risks were fully described to the subjects. The study was approved by the University's human ethics committee.
Experimental Protocol
During the 24-h period before each trial the subjects abstained from caffeine and alcohol. About 2 h before arrival at the laboratory subjects ate a light breakfast (toasted bread and juice). Experiments began at about 8:00 AM and consisted of about 1 h of preparation and 5 h of data collection.Before insertion of catheters, the skin was infiltrated with 0.5 ml of 2% Xylocaine (lidocaine) without epinephrine (Astra Pharma, Mississauga, ON). A brachial artery and an antecubital vein (opposite arm) extending into the deep tissues were catheterized percutaneously with 20-gauge 1.25-in.-long Teflon catheters (Becton-Dickenson Angiocath; Baxter, Mississauga, ON). The patency of the catheter was maintained using a slow drip (200 µl/min) of isotonic saline.
After insertion of catheters the subjects sat quietly for 30 min.
Baseline (control) blood samples were obtained at 10 and 30 min
(experiment time 
20 and 0 min, respectively).
After this 30-min period (experiment time 0 min), the subjects
began ingestion of 3.57 mmol/kg body mass
KHCO3 or
NaHCO3 as a 600 mosmol/l flavored solution (Kool Aid with Nutrasweet). The ~920 ml were ingested in six
aliquots over six sequential 10-min periods. The subjects were observed
for a further 210 min in the postingestion period.
Safety Precautions
Elevation of [K+] to 8.0 mM or evidence of cardiac abnormalities such as tented T waves were used as indicators for intervention (16, 36). During and after KHCO3 ingestion, plasma [K+] was measured at 10-min intervals. A three-lead electrocardiogram (ECG) was also monitored continuously.An appropriate ingestion protocol for KHCO3 was established using a pilot study using two subjects. The criteria were to induce a large and rapid increase in plasma [K+] within safe limits (peak plasma [K+] at or below 7 meq/l with no ECG abnormalities). The dose of KHCO3 (3.57 meq K+/kg body mass) was the same as that shown to be of ergogenic effect with NaHCO3 (20). A 30-min ingestion period resulted in a pronounced and long-lasting hyperkalemia; however, plasma [K+] reached 6-8 meq/l for 1-2 h and was associated with a tenting of T waves. Consequently, the ingestion period was increased to 60 min, and this resulted in a slower rate of increase of plasma [K+] without tenting of T waves in either subject. In the subsequent experiments, one of the six subjects had pronounced tenting of T waves after 40 min of ingestion of the KHCO3 solution and was promptly treated with intravenous glucose and Ca2+ (36). This resulted in immediate reversal of T wave forms and rapid normalization of plasma [K+]. This individual's data are excluded from the experiment. As a consequence, the results include data from the five subjects that fully completed both protocols.
Measurements and Analysis
Arterial and venous blood were sampled simultaneously at 10- to 30-min intervals in 10-ml heparinized syringes (10 IU lithium heparin/ml; Sarstedt, Numbrecht, Germany). The sample was immediately analyzed in duplicate for Hct, blood gases (PCO2, PO2), plasma ions [H+ (from pH electrode), HCO3 (calculated),
Na+,
K+,
Ca2+,
Cl], and glucose
using ion and metabolite selective electrodes (Nova Statprofile 5; Nova
Biomedical, Waltham, MA), where
Ca2+ is ionized
Ca2+ concentration
([Ca2+]) normalized to
a plasma pH of 7.40. The remaining blood was transferred into plastic
tubes and centrifuged at 13,000 g for 5 min; the plasma portion was removed and stored on ice. Plasma (200 µl) was deproteinized in 6% perchloric acid (400 µl), and the
extract was analyzed for lactate by enzymatic fluorometric analysis
(5). A clinical refractometer (Atago model 331) was used to measure
plasma protein concentration ([PP]).
Calculations
Plasma volume and ECFV. The initial plasma volume (PV) was estimated as 38 ml/kg body mass (22), with ECFV taken as five times the PV (27); the interstitial fluid volume (ISFV = ECFV PV) was thus four times the PV.
The percent change in PV (%
PV) was calculated using
[PP]
![%&Dgr;PV<SUB>pp</SUB> = 100 × ([PP]<SUB>i</SUB> − [PP]<SUB><IT>t</IT></SUB>)/[PP]<SUB><IT>t</IT></SUB>](/content/vol276/issue1/fulltext/R32/img001.gif)
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(1) |
PVPP with the estimated
initial PV. The plasma compartment was assumed to be in or near
electrochemical and physicochemical equilibrium with other ECF
compartments and was taken as representative of the entire ECF compartment.
A discrepancy in the value for %PV calculated using Hct
(%PVHct) with that of
%PV calculated using PP
(%PVPP) was used to
determine if red blood cells gained or lost volume (12, 19) as a result
of NaHCO3 or
KHCO3 ingestion. The
%PVHct was calculated as (14)
![%&Dgr;PV<SUB>Hct</SUB> = 100 × [(Hct<SUB>i</SUB> − Hct<SUB><IT>t</IT></SUB>)/Hct<SUB><IT>t</IT></SUB>]/[1 − (Hct<SUB><IT>t</IT></SUB>/100)]](/content/vol276/issue1/fulltext/R32/img002.gif)
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(2) |
PV only when there has been no change in hemoglobin concentration or in red
blood cell mean corpuscular volume (MCV; see Refs. 14 and 19).
Therefore a discrepancy between
%PVHct and
%PVPP may be taken as evidence
of a change in MCV.
Estimates of the total content of electrolyte in the plasma and ECF compartments were obtained from the product of the arterial plasma ion concentration and the PV or ECFV, respectively. This was necessary to properly assess ion balance due to simultaneous changes in PV and ion concentrations that occurred in response to the ingestion of solutions.
The cumulative net flux of Na+ (in the NaHCO3 trial) and K+ (in the KHCO3 trial) across the tissues of the forearm was used to estimate whole body skeletal muscle Na+ or K+ flux
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(3) |
![= <LIM><OP>∫</OP><LL><IT>t</IT></LL><UL>0</UL></LIM> (a-v[ion]) × <A><AC>Q</AC><AC>˙</AC></A> × 0.45BM × <IT>t</IT>](/content/vol276/issue1/fulltext/R32/img004.gif)
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is a mean tissue perfusion
rate of 0.02 l · min1 · kg1
(11), skeletal muscle mass was taken as 45% of total body mass (BM, in
kg; see Ref. 10), and t is total time
in minutes. This recognizes that the skeletal muscle component of the
forearm is dominant with respect to gas (29) and ion (9) exchange.
The plasma [SID] was calculated as the sum of the plasma strong cation concentrations minus the sum of the strong anion concentrations (34, 35)
![[SID] (meq/l) = ([Na<SUP>+</SUP>] + [K<SUP>+</SUP>]](/content/vol276/issue1/fulltext/R32/img005.gif)
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(4) |
![+ [Ca<SUP>2+</SUP>]) − ([Cl<SUP>−</SUP>] + [lactate<SUP>−</SUP>])](/content/vol276/issue1/fulltext/R32/img006.gif)
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] is
lactate ion concentration. Plasma pH was converted to
[H+] by logarithmic
transformation. In addition, plasma
[H+] was calculated
according to the following equation consistent with mass action
equilibria and electroneutrality of solutions (34, 35)
![[H<SUP>+</SUP>]<SUP>4</SUP> + (K<SUB>A</SUB> + [SID]) × [H<SUP>+</SUP>]<SUP>3</SUP>](/content/vol276/issue1/fulltext/R32/img007.gif)
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(5) |
![+ [([SID] − [A<SUB>Tot</SUB>])(K<SUB>A</SUB>) − (K<SUB>C</SUB> × P<SC>co</SC><SUB>2</SUB> + K′<SUB>W</SUB>)] × [H<SUP>+</SUP>]<SUP>2</SUP>](/content/vol276/issue1/fulltext/R32/img008.gif)
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![− [(K<SUB>C</SUB> × P<SC>co</SC><SUB>2</SUB> + K′<SUB>W</SUB>)(K<SUB>A</SUB>) + (K<SUB>3</SUB> × K<SUB>C</SUB> × P<SC>co</SC><SUB>2</SUB>)] × [H<SUP>+</SUP>]](/content/vol276/issue1/fulltext/R32/img009.gif)
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7 eq/l (34, 35),
KC = 2.46 × 1011 eq/l (34, 35),
K3 = 6.0 × 1011 eq/l (15), and
K'W = 4.4 × 1014 eq/l (18).
Plasma ATot concentration
([ATot]) was
calculated as [PP] × 2.85; the empirical factor of
2.43 (34, 35) used previously (23, 25) yielded consistently low
[ATot] compared with
those calculated from [SID],
PCO2, and
[H+]
(Eq. 5). The reason for the
discrepancy arose primarily from the inclusion of plasma
[Ca2+] in the
calculation of [SID], thus resulting in a higher
[SID] (by ~3 meq/l) than if
[Ca2+] was omitted.
Plasma [Ca2+] was
included in the calculation of [SID] because it can change and because of its interaction with PPs, the
[ATot] portion of plasma. In addition, in the present study, the nonfasted state of the
individuals may have resulted in lower plasma free fatty acid
concentrations that allowed for greater binding of
H+ to PPs (33). Unmeasured weak
anions did not have a significant effect on the physicochemical
assessment of acid-base balance. The ionized form of
[ATot],
[A], was 18.0 ± 0.7 meq/l when calculated using [SID] [HCO3] [A] = 0 (34),
very similar to that calculated using measured
[H+], with
[SID], and PCO2
(Eq. 5).
Statistics
All reported values are means ± SE. A two-way analysis of variance with repeated measures was employed for assessment of dependent variables with respect to treatment and time. When a significant F ratio was obtained, the Student-Newman-Keuls method was used to compare the means. Statistical significance was accepted at P
0.05.
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RESULTS |
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Top
Abstract
Introduction
Methods
Results
Discussion
References
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PP and Change in PV
With NaHCO3 ingestion, [PP] remained unchanged until 120 min (Table 1). A subsequent decrease in [PP] from 135 to 270 min represented a 115- to 210-ml increase in PV (Fig. 1). In the KHCO3 trial, arterial and venous [PP] were both increased between 60 and 270 min (Table 1). The corresponding decreases in PV were 296 ± 89 ml (60 and 210 min) and 474 ± 59 ml at 120 min (Fig. 1). By 240 min, [PP] and %PV were not different from initial baseline values.
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The magnitude of changes in arterial and venous (not shown) Hct were
quantitatively different from that of [PP] (Table 1), allowing changes in MCV to be estimated from the difference between %PVPP and
%PVHct. Between 90 and 270 min
in the NaHCO3 trial, the change
() in PVHct increased by 356 ml
(12%); this was about twofold greater than that calculated using
[PP], indicating a decrease in red blood cell MCV
equivalent to ~180 ml for the entire red blood cell compartment. In
contrast, in the KHCO3 trial,
between 50 and 270 min, PVHct
decreased by 235-415 ml; this was 60-100 ml less than that
calculated using [PP], indicating an increase in red blood
cell MCV.
In the NaHCO3 trial, PV, estimated ISFV, and ECFV were all elevated at 135 min (Table 2). However, in the KHCO3 trial, the 445 ± 89 ml decrease in PV at 135 min represented a 2.5-liter decrease in ECFV and a 2.1-liter decrease in ISFV (Table 2); by 270 min, ECFV had recovered 70% of the deficit that existed at 135 min.
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K+
In the NaHCO3 trial, arterial and venous plasma [K+] decreased below initial values by 165 min and remained depressed until the end of the experiment (Fig. 2A and Table 3). Between 30 and 70 min, there was a short-lived net K+ efflux from the arm (Fig. 2B). This a-v[K+] was short lived and was fully abolished by 110 min. No detectable change in plasma K+ content was observed (Fig. 2C).
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With KHCO3 ingestion, arterial and
venous [K+] increased
to 7.17 ± 0.13 meq/l at 110 min and to 6.36 ± 0.19 meq/l at 135 min, respectively (Fig. 2A and Table
3). The decrease in PV (Fig. 1) accounted for 35-40% of the
increase in plasma
[K+] from 50 min
onward (Fig. 2A). The remainder of
the increase in plasma
[K+] and content (Fig.
2C) must therefore have resulted
from the net movement of K+ into
the ECF compartments from the intestinal tract. The net amount of
K+ transported into the plasma
compartment at 100 min was estimated to be 5.5 meq or ~27 meq for the
entire ECF. Arm K+ extraction
between 30 and 240 min (Fig. 2B)
resulted in a peak a-v[K+] of 1.22 ± 0.25 meq/l at 70 min. Assuming a forearm blood flow of ~20
ml · min1 · kg1
(11), this represents a net K+
influx of 24.4 µeq · min1 · kg1
or 66 meq/h for 45 kg of mass (10) capable of exchanging
K+. At the end of the experiment
only 3% of the ingested K+ was
estimated to be in the ECF compartment, whereas
K+ extraction by the tissues
accounted for 35% of ingested K+
(Table 4).
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Na+
In the NaHCO3 trial, arterial plasma [Na+] was increased between 50 and 90 min (Fig. 3A), with no change in venous plasma [Na+] (Table 3) and no significant net uptake or release of Na+. The increase in plasma Na+ content between 80 and 270 min (Fig. 3B) accounted for 56% of ingested Na+ (Table 4) and was coincident with the increase in PV (Fig. 1).
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In the KHCO3 trial, arterial (Fig. 3A) and venous (Table 3) plasma [Na+] decreased by ~3 meq/l between 100 and 270 min. The decrease in plasma Na+ content between 60 and 240 min (Fig. 3B) was largely accounted for by the decrease in PV (Fig. 1).
Cl
] were
similar and showed no significant change over time.
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In the KHCO3 trial, there was no
net release or uptake of
[Cl]. The
decrease in arterial plasma
[Cl] (Fig.
4A and Table 3), together with the
decrease in PV, resulted in a significant decrease in plasma
Cl content between 60 and
210 min; plasma Cl content
recovered by 240 min (Fig. 4B).
Ca2+, Lactate, and Glucose
In both trials, arterial and venous plasma [Ca2+] did not change with time, and there was no difference between trials: range 2.36-2.53 meq/l.In the NaHCO3 trial, arterial
plasma
[lactate]
decreased significantly from 0.7 ± 0.2 meq/l preingestion to 0.5 ± 0.2 meq/l at 90 min postingestion and thereafter remained
unchanged. In the KHCO3 trial,
[lactate] did
not change with time. In both trials, a net negative
a-v[lactate] of
~0.2 meq/l remained unchanged over time. There was no effect of
treatment on plasma glucose concentration ([glucose];
remained at 5.8 ± 0.3 mmol/l), and, in both trials, arterial plasma
[glucose] was greater than venous (not shown) by ~0.3
mmol/l.
Acid-Base Status
Origins of change in [H+]. Plasma [H+] calculated from the independent variables [SID], PCO2, and [ATot] was not different from that calculated from measured pH; the difference between the means averaged 0.7 ± 0.02 neq/l for both trials combined. This allowed us to evaluate the physicochemical origins of the changes in plasma [H+] from changes in the independent variables [SID], [ATot], and PCO2.
The time courses of measured [H+] and calculated arterial plasma [H+], when each of the independent variables of acid-base control were changed alone, are shown in Fig. 5. For example, the changes in [SID] were applied while keeping [ATot] and PCO2 constant at time 0 values, with the process repeated for the other independent variables.
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]
(2.5 meq/l; Fig. 4A).
Arterial PCO2 increased gradually during the ingestion period by 5.6 ± 1.3 mmHg at 90 min (Fig. 7B). The increase in
PCO2 alone would have produced an increased [H+] (Fig.
5A); however, this effect (i.e.,
measured [H+]) was
exceeded by the alkalinizing effect of increased [SID]. Arterial plasma [ATot]
did not change until after 120 min, when it remained 1 meq/l lower than
initial for the remainder of the experiment (Fig.
7C). This change was too small to
contribute significantly to changes in
[H+] over time (Fig.
5A). An absence of change in venous
plasma [SID] indicated that the arm modified the ion
composition of the perfusing plasma. Venous
PCO2 increased by 10.3 ± 1.7 mmHg
at 80 min (not shown), resulting in a trend
(P = 0.073) toward a more negative
a-vPCO2 (Fig. 6).
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]
(2 meq/l). There was a rapid, 2 meq/l increase in arterial plasma [ATot] by 60 min, with an additional 1 meq/l increase by 135 min (Fig.
7B); this was due to the decrease in
PV. The increase in
[ATot] alone would
have increased [H+] by
3.9 ± 0.8 neq/l at 120 min (Fig.
5B). In both trials, plasma a-v[ATot] was not
different from zero and did not change over time. Neither arterial,
venous, nor a-vPCO2 changed with time
(Fig. 7C), so
PCO2 did not contribute to changes in
[H+] in the
KHCO3 trial (Fig.
5B). As in the
NaHCO3 trial, venous plasma
[SID] did not change, indicating that the tissues modified plasma ion composition.
Origins of change in
[HCO3].
In the NaHCO3 trial, arterial
plasma [HCO3] reached a
peak of 32.7 ± 0.8 meq/l at 90 min compared with an initial value
of 26.0 ± 0.4 meq/l (Fig.
8A).
Venous plasma [HCO3] was
consistently greater (by 2-3 meq/l) than arterial, and there was
no change in a-v[HCO3]
with time (not shown). The increase in [SID] was the
primary (and nearly sole) determinant for the rise in
[HCO3]; changes in
PCO2 and
[ATot] alone or in
combination did not significantly influence changes in
[HCO3].
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3] had increased by
~5 meq/l between 80 and 100 min (Fig.
8B). Venous plasma
[HCO3] was consistently
greater (by 2-3 meq/l) than arterial, with no change in
a-v[HCO3] with time (not
shown). The increase in [SID] was the primary determinant for the increase in
[HCO3]. The increase in [ATot] contributed to
a decrease in [HCO3], and
PCO2 had no effect.
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DISCUSSION |
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Top
Abstract
Introduction
Methods
Results
Discussion
References
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The present study found that the forearm, of which skeletal muscle is dominant with respect to fluid and ion exchange, modified the ionic and acid-base composition of perfusing blood during and after NaHCO3 and KHCO3 ingestion. Both NaHCO3 and KHCO3 produced a metabolic alkalosis; however, differences in the magnitude and time course reflected different origins of the fluid and ion disturbance, depending on whether the cation was Na+ or K+. These differences are associated with different processes for the intestinal transport of water, Na+ and K+, and their differential distribution in extra- and intracellular fluid compartments. Particularly noteworthy in the KHCO3 trial was the >1 meq/l reduction in plasma [K+] that occurred as blood perfused the tissues from the arterial to the venous side of the circulation. It has been shown that tissue ion exchange processes effectively regulated plasma ion composition and acid-base state and are of physiological importance to the acute correction of plasma fluid and ion disturbances.
Methodology and Limitations
Blood flow, perfused muscle mass, gastric emptying rate, and intestinal water and ion absorption rates were not measured. The estimates of tissue water and ion balance (Tables 2 and 4) are based on the assumption that the majority of forearm ion exchange is dominated by skeletal muscle (6, 9) and that fluid and ionic equilibria were at least approached among ECF compartments. The quantity of ingested water and electrolyte remaining in the gastrointestinal tract at any point in time was estimated based on the time course of changes in plasma/ECF water and ion contents and plasma a-v[ion] across the arm.It is relevant that if only antecubital venous blood, and not arterial blood, had been sampled, the interpretation of the effects of NaHCO3 and KHCO3 loading on systemic function would be markedly different from that presented here. This is because the magnitude and time course of changes in venous plasma often varied from that of arterial plasma due to the rapidity of gas and ion exchange processes in skeletal muscle.
Plasma Acid-Base Balance
Ingestion of both NaHCO3 and KHCO3 resulted in a persistent arterial metabolic alkalosis. However, compared with the NaHCO3 trial, the alkalosis in the KHCO3 trial was slower (by ~30%) to occur and was lower in magnitude of decrease in [H+] by ~30%. This can be attributed to notable differences in the physicochemical origins of the decrease in plasma [H+] and increase in [HCO3]. In both trials,
the increase in arterial plasma [SID] was the primary
determinant of the decrease in
[H+] and increase in
[HCO3]. In general, strong basic cations were only 50-60% responsible for the increase in plasma [SID], with the balance contributed by 2 to 3 meq/l
decreases in plasma
[Cl]. How the
increase in arterial plasma [SID] was achieved in the two
trials was markedly different. In the
NaHCO3 trial, increases in plasma
[Na+] and decreases in
plasma [Cl]
contributed equally to the increase in [SID]. In the
KHCO3 trial, the increase in
arterial plasma [SID] was due mainly to the combination of
increased plasma [K+]
and decreased
[Cl].
Increased PCO2, in the
NaHCO3 trial, had an acidifying
effect that partially offset the decrease in
[H+] and increase in
[HCO3] that would have
been induced by increases in [SID] alone. In the
KHCO3 trial the more modest
increases in arterial plasma
[HCO3] were not associated
with increases in PCO2. It is
speculated that this may have been associated with a measurably greater
rate of ventilation and 
CO2
in the KHCO3 trial compared with
the NaHCO3 trial (unpublished observation).
In the KHCO3 trial, large and
rapid increases in
[ATot] had an
acidifying effect that contributed to partially offsetting the
[SID]-induced decrease in
[H+] and increase in
[HCO3]. This, however, was not evident in the NaHCO3 trial.
Thus a similar picture of acid-base disturbance in the two trials, with
respect to plasma [H+]
and [HCO3], are seen to
have markedly different origins with respect to the independent
physicochemical determinants of acid-base control.
Water Balance
The main determinants of changes in PV include the magnitude and rate of intestinal net water flux, the distribution of water among intracellular, interstitial, and vascular compartments, and excretion of water and ions by the kidneys. Changes in PV are important because they influence PP, ion, and acid-base status and, ultimately, cellular and whole organism function.In both trials the subjects ingested solutions that had an osmolality
~570 mosmol/kgH2O and were thus
hypertonic to body fluids. Although net intestinal water flux is
passive, it is coupled to net Na+,
but not K+, transport (21), such
that the intestinal epithelium is able to transport fluid against an
osmotic gradient (13). In the NaHCO3 trial, there was no
evidence for net water movement into the gastrointestinal tract since
PV was initially unchanged and subsequently (after 120 min) was
observed to increase. The rate of water absorption after the ingestion
of isotonic saline-HCO3 (150 meq/l
Na+, 120 meq/l
Cl, 30 meq/l
HCO3) has been reported to be 4.20 ml · h1 · cm1
of small intestine (32). This rate of water absorption (assuming 100 cm
of jejunum) would have moved 1,890 ml of fluid, or twice the ingested
volume, during the 270-min experiment. Therefore, it is probable that
the entire volume of ingested
NaHCO3 was absorbed in the present
study. At the end of the experiment, the body was in positive water
balance by 715 ml, with the ECF compartment in positive balance by 954 ml (Table 2), suggesting a net loss of intracellular fluid volume
(ICFV) of ~240 ml. This is consistent with the estimated
decrease in red blood cell MCV in this trial. Correction of the fluid
disturbance occurred primarily by increased renal excretion of water,
Na+, and base equivalents by the
kidneys (unpublished observation).
In the KHCO3 trial, the 15% decrease in PV within 70 min after completion of ingestion (at 120 min) represented a net loss of ~2 liters of water from the ECF into the gastrointestinal tract and possibly other tissues. Although net water flux into tissues was not detectable, the change in PV estimated from Hct underestimated that calculated from [PP], suggesting that there was a net increase in red blood cell MCV.
The proximal portion of the duodenum is highly permeable to water, and
this allows for dilution of concentrated solutions in the proximal
small intestine, thus facilitating absorption in the distal regions
(17). In the KHCO3 trial it is
suggested that the initial rapid decrease in PV was due to the net
movement of water and Na+ (see
below) into the proximal duodenum. This appeared to be followed by
elevated rates of net water, Na+,
and K+ absorption in the distal
small intestine, consistent with the gradual recovery of PV and
subsequent diuresis, natriuresis, and kaliuresis (unpublished
observations). Complete intestinal absorption of the ingested volume
may have occurred by 270 min. In support, ingestion of 5 mmol/l KCl
with 95 mmol/l NaCl and 45 mmol/l
NaHCO3 in humans resulted in a net
rate of water absorption of 4-5
ml · h1 · cm1
of small intestine (21). In the present study, the minimum mean jejunal
water absorption rate required to achieve full absorption of the
ingested KHCO3 solution (915 ± 59 ml) was estimated to be 2.6 ml · h1 · cm1,
~60% of the value obtained by Hicks and Turnberg (21).
Na+ Balance
In the NaHCO3 trial, the increases in plasma Na+ content and PV implied a rapid distribution of absorbed Na+ and water throughout the ECF. Correction of this expanded ECF compartment is consistent with the increased renal excretion of water and Na+ (unpublished observation). In this trial, it is probable that all of the ingested Na+ was absorbed. In support, Sladen and Dawson (32) reported jejunal Na+ absorption rates of 0.73 meq · h1 · cm1
in humans administered isotonic, glucose-free (as in the present study)
saline-HCO3 (150 mM
Na+, 120 mM
Cl, 30 mM
HCO3). At these rates, with a proximal small intestine 100 cm long (39), 328 meq of
Na+ would be absorbed in 270 min,
greater than the 280 meq of Na+
ingested in the present study.
In contrast to the NaHCO3 trial,
KHCO3 ingestion resulted in a
hyponatremia that appeared to be due to net water,
Na+, and
Cl secretion in the
gastrointestinal tract (17) and to increased renal
Na+ excretion (unpublished
observations); there was no evidence of net
Na+ movement into cells.
K+ Balance
In the KHCO3 trial, 60-65% of the increase in plasma [K+] originated from a rapid increase in intestinal K+ absorption, whereas the decrease in PV accounted for 35-40% of the increases in plasma and ECF K+ contents and plasma [K+]. Correction of elevated plasma and ECF [K+] occurred by increased tissue K+ extraction (accounting for 37% of ingested K+; Table 4) and increased renal K+ excretion [accounting for 93 ± 16 meq (34%) of ingested K+; unpublished observations].It is suggested that all, or at least a majority, of ingested
K+ was absorbed from the intestine
by the end of the experiment. Duodenojejunal
K+ transport is dependent on the
electrochemical potential difference for
K+ between plasma and intestinal
lumen and is associated with the absorption of
Na+, water, and other nutrients
(3, 17, 31). Passive K+ absorption
rates of ~0.02
meq · h1 · cm1
have been reported from proximal jejunum after ingestion of a solution
consisting of 5 mM KCl with 45 mM
NaHCO3 and 95 mM NaCl (21).
However, in the present study, the electrochemical potential difference
for K+ across the small intestine
would initially have been large, as ingested solution
[K+] was 278 meq/l,
strongly favoring net K+
absorption. If we assume a K+
absorption rate in our KHCO3
trials of 0.02 meq · h1 · cm1
(from Ref. 21), then only ~9 meq of
K+ would have been absorbed by the
end of the experiment. In contrast, estimated initial net
K+ transport rates in the jejunum
and ileum, from an assumed mean luminal
[K+] of 150 meq/l
(assumes achievement of osmotic equilibrium between intestinal lumen
and plasma), are ~15 (jejunal) and 12 (illeal) meq · h1 · cm1
(3) or, on average, ~1,300 meq/h. At this rate, the ingested K+ would have been absorbed in
just over 11 min (280 meq, 100-cm segment). Because luminal
[K+] certainly
decreased rapidly with time, such high rates would not be maintained.
For complete absorption of the ingested
K+ to have occurred by 270 min,
the average net rate of K+
absorption would have been 0.8 meq · h1 · cm1,
markedly less than the estimated peak rates of 12-15
meq · h1 · cm1.
Skeletal muscle is recognized for its involvement in the extrarenal regulation of plasma [K+] via modulation of Na+-K+-ATPase activity (6, 9). In the present study, the widened a-v[K+] of 1.22 meq/l at 70 min represents an estimated peak K+ absorption rate of 66 meq/h (see RESULTS). The short-term regulators of Na+-K+-ATPase activity include intracellular [Na+], extracellular [K+], plasma insulin, and plasma catecholamines (9); however, catecholamines do not change in response to NaHCO3 ingestion (7). Intracellular [Na+] would be low under the conditions of this study, and this would prevent marked increases in Na+-K+-ATPase activity (9). The 3 meq/l increase in arterial plasma (and muscle ECF) [K+] should, nonetheless, have resulted in increased flux of K+ into muscle. Aldosterone is known to be involved in the long-term control of skeletal muscle Na+-K+-ATPase activity (6). In the KHCO3 trial, an increased plasma aldosterone (from 0.2 ± 0.04 to 1.2 ± 0.21 nmol/l at 90 min, unpublished observations) paralleled the increase in plasma [K+]. However, aldosterone may have contributed little, if any, to the widening plasma a-v[K+] as peak plasma aldosterone occurred between 90 and 150 min, whereas peak plasma a-v[K+] occurred at 70 min, and at 130 min plasma a-v[K+] was not significantly elevated. Another possibility is that increases in plasma insulin may have increased Na+-K+-ATPase activity (9) as a result of a plasma [K+]-induced release of pancreatic insulin (6). However, it is unlikely that plasma insulin increased in this study as there was no decrease in plasma [glucose], nor an increase in a-v[glucose], in either trial. It is concluded that the primary stimulus for the widened a-v[K+] (increased Na+-K+-ATPase activity) was the increase in arterial plasma and muscle ECF [K+].
Given the presence of the K+ control systems, it is interesting that plasma [K+] increased to >7 meq/l and remained elevated for an extended period. The body possesses an abundance of Na+-K+ pumps that, in inactive skeletal muscle, operate at only 10-15% of their capacity (9). The total skeletal muscle pool has a maximal capacity for K+ reabsorption of ~125 meq/min or 7,500 meq/h (9). At this rate the K+ ingested in the KHCO3 trials could be taken up in 135 s. The limited use of the Na+-K+-ATPase reserve capacity for K+ regulation probably reflects a high intracellular [K+] and a low intracellular [Na+] in the tissues, preventing larger increases in Na+-K+-ATPase activity.
In the NaHCO3 trial, a negative a-v[K+] between 30 and 70 min was due to an increase [not significant (NS)] in venous plasma [K+] and a decrease (NS) in arterial plasma [K+] and plasma K+ content. It has been suggested (1, 2) that the alkalosis resulting from NaHCO3 increases intracellular [Na+] through exchange of intracellular H+ for extracellular Na+ via the Na+-H+ antiporter (4). Increased intracellular [Na+] in turn stimulates Na+-K+-ATPase activity to reduce extracellular [K+] (hypokalemia) and increase intracellular [K+] (8). Although the clinical efficacy of intravenous NaHCO3 therapy to attenuate a developing hyperkalemia is well established (36), only a very modest hypokalemia developed after 160 min in the present study. Measurement of a-v[K+] across the arm showed no evidence of increased net movement of K+ into the tissues of humans having ingested NaHCO3.
Perspectives
The majority of studies have attributed the ergogenic effect to NaHCO3 loading to the ensuing alkalosis. Purportedly, an increased ability of muscle to produce force results from 1) an enhanced use of the CO2-HCO3
system to buffer protons released to the ECF at increased rates from
contracting skeletal muscle and 2)
an attenuated rate and magnitude of increase in muscle intracellular
[H+] (20, 26).
However, the present study has shown that other fluid and ion shifts
may also be important. NaHCO3
loading was associated with an increased ECFV that could enhance
cardiovascular function and thermoregulatory cooling (17, 30).
Furthermore, in both the NaHCO3
and KHCO3 trials, the primary
determinant of plasma alkalinization was the increase in plasma
[SID]. As such, changes in plasma strong ion concentrations
play an important role in the development of, and recovery from,
acid-base disturbances. Lactate, an important
strong acid anion in exercise situations (23, 25), is released at
increased rates from skeletal muscle under alkalotic conditions (see
Ref. 20), and an elevated [SID] before the onset of
exercise may partially counteract the rise in plasma lactate
concentration, attenuating acidification of both the ECF and
intracellular fluid compartments.
The markedly different whole body responses to ingested
NaHCO3 and
KHCO3 in humans at rest are
attributed to the primarily extracellular distribution of ingested
Na+ and to the primarily
intracellular distribution for K+.
The differential distribution and renal handling of the water and
cation loads influenced the magnitude and time course of the acid-base
disturbances. NaHCO3 ingestion was
characterized by increases in plasma and extracellular water associated
with the increase in
[Na+] and
Na+ content. The increase in
plasma [Na+] and
decrease in plasma
[Cl] combined
to increase plasma [SID], which was the major contributor to the plasma alkalosis. The ingestion of
KHCO3 resulted in a significant
hemoconcentration, probably associated with a net water flux into the
intestinal lumen early during the ingestion period. Intestinal
K+ absorption contributed to the
marked increase in plasma
[K+], with
K+ extraction by skeletal muscle
accounting for 37% of ingested K+
by 270 min. The metabolic alkalosis that occurred with
NaHCO3 ingestion was primarily the
result of increased [SID], but due primarily to increases
in plasma [K+] and
secondarily to decreases in plasma
[Cl].
| |
ACKNOWLEDGEMENTS |
|---|
This study was supported by the Natural Sciences and Engineering Research Council of Canada and the Medical Research Council of Canada.
| |
FOOTNOTES |
|---|
G. J. F. Heigenhauser is a Career Investigator with the Heart and Stroke Foundation of Ontario. L. C. Lands is a Chercheur-clinicien with the Fonds de la Recherché en Santé du Quebec.
Address for reprint requests: M. I. Lindinger, Dept. of Human Biology & Nutritional Sciences, Univ. of Guelph, Guelph, ON, Canada N1G 2W1.
Received 25 November 1997; accepted in final form 11 August 1998.
| |
REFERENCES |
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Top
Abstract
Introduction
Methods
Results
Discussion
References
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) and
KHCO3 (
) ingestion. The
KHCO3 trial data are significantly
different from the NaHCO3 trial
data. Values are means ± SE for n = 5 subjects. Hatched bar indicates 60-min ingestion period.
* Mean significantly different
(P < 0.05) from
time 0. ** Mean significantly
different from peak or nadir.
,
calculated arterial plasma
[H+] when only
PCO2 changes and strong ion
difference ([SID]) and total concentration of weak acids
and bases ([ATot]) are
kept constant; 
, calculated arterial plasma
[H+] when only
[ATot] changes and
[SID] and PCO2 are kept
constant; 
, calculated arterial plasma
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and [ATot] are kept
constant. Hatched bar indicates 60-min ingestion period. * Mean
significantly different (P < 0.05)
from time 0.
