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Division of Comparative Physiology and Biochemistry, Society for Integrative and Comparative Biology The Effect of Temperature Acclimation and Adrenaline on the Performance of a Perfused Trout Heart Author(s): M. S. Graham and A. P. Farrell Source: Physiological Zoology, Vol. 62, No. 1 (Jan. - Feb., 1989), pp. 38-61 Published by: The University of Chicago Press. Sponsored by the Division of Comparative Physiology and Biochemistry, Society for Integrative and Comparative Biology Stable URL: http://www.jstor.org/stable/30159997 . Accessed: 19/11/2014 15:54 Your use of the JSTOR archive indicates your acceptance of the Terms & Conditions of Use, available at . http://www.jstor.org/page/info/about/policies/terms.jsp . JSTOR is a not-for-profit service that helps scholars, researchers, and students discover, use, and build upon a wide range of content in a trusted digital archive. We use information technology and tools to increase productivity and facilitate new forms of scholarship. For more information about JSTOR, please contact [email protected]. . The University of Chicago Press and Division of Comparative Physiology and Biochemistry, Society for Integrative and Comparative Biology are collaborating with JSTOR to digitize, preserve and extend access to Physiological Zoology. http://www.jstor.org This content downloaded from 206.87.119.142 on Wed, 19 Nov 2014 15:54:21 PM All use subject to JSTOR Terms and Conditions 38 The Effect of Adrenaline of a Perfused Temperature Acclimation on the Trout and Performance Heart M.S. Graham* A.P.Farrell of BiologicalSciences,SimonFraserUniversity, Department BritishColumbiaV5A1S6 Burnaby, Accepted5/24/88 Abstract Cardiac performance was examined with in situ perfused trout hearts at two acclimation temperatures, 5 C and 15 C. In series I, adrenaline-free perfusion and a cumulative dose response up to 1 jgmol adrenaline - L-' was examined. In series II, tonic adrenergic stimulation (5 nmol . L-) and a cumulative dose response up to 50 nmol - L-1 was examined Tonic adrenergic stimulation was importantfor chronotropic and inotropic stability, especially at5 C. Heart rate and maximum cardiac output were significantly higher at 15 C than at5 C. Maximum stroke volume at5 C was the same as or greater than the maximum stroke volume at 15 C Adrenergic stimulation produced quantitatively differentpositive chronotropic and inotropic effects at both temperatures andpartially compensatedfor the direct efect of temperature; the chronic Q.o valuesfor heart rate and maximum cardiac output were 1.30-1.40. Trout acclimated to 5 C had a relatively larger ventricle mass, which permitted a higher absolute stroke work at 5 C than at 15 C Introduction When faced with a change in watertemperature,fish can either compensate for the temperaturechange, conform to it, or avoid the thermal effects by modifying their behavior (Precht 1958). In terms of cardiacfunction, temperaturedirectly affects the intrinsic properties of the heart and indirectly affectscardiacfunction throughtemperature-relatedmodificationsto extrinsic controls (Randall 1970; Seibert 1979; Wood, Pieprzak,and Trott 1979; * Current 3X8Canada. British P.O.Box3232,Vancouver, address: Vancouver Public Columbia, V6B Aquarium, ofChicago. 1989.C 1989byTheUniversity Zoology Physiological 62(1):38-61. Allrights reserved. 0031-935X/89/6201-87112$02.00 This content downloaded from 206.87.119.142 on Wed, 19 Nov 2014 15:54:21 PM All use subject to JSTOR Terms and Conditions Acclimation intheTrout Heart 39 Temperature TABLE1 Morphometric and biologic information ExperimentalSeries Total Body Mass(g) Ventricle Mass(g) Ventricle: Body-Mass Sex Ratio Ratio(%) (M:F) 622 .64a .103a (14.2) (.040) (.0051) 561 (18.6) .44b .078b (.046) (.0055) 596 .70a .117 (40.8) (.096) (.0146) 531 (34.8) .42b (.031) .078b (.0025) 8:1 485 .38b .070b 3:1 (53.9) (.085) (.0081) Series I (5 C, N= 11) 10:1 Series I (15 C, N= 7) Series II (5 C, N= 6) Series II (15 C, N= 9) Time trials (15 C, N= 4) 4:3 5:1 Note.Allvaluesexceptthosefor"Ventricle:Body-Mass Ratio"aremeans(SEM)forN animalsin eachseries.Significant differences(P < .05)forventriclemassand experimental ratioareindicatedbymeanvalueshavinga differentlettersuperscript. ventricle:body-mass Farrell1984). While the direct effects of temperaturetend to suppress cardiac activity (negative chronotropyand inotropy), adrenergic stimulation tends to increase cardiac activity (positive chronotropyand inotropy). In view of these antagonisticactions, we examined whether adrenergicstimulation of the heartwas an importantmechanismto compensate for the direct effects of temperature. Adrenaline is found in the blood of resting trout (Butler, Metcalfe, and McGinley1986; Primmettet al. 1986;Milliganand Wood 1987) and is more effective than noradrenalineas a cardiacstimulant (Nilsson 1981, 1983;Ask 1983;Farrell,MacLeod,and Chancey 1986). Withstressfulexercise, plasma adrenalinelevels rise from 1-5 nmol - L-1to 35-50 nmol - L-1in trout(Primmett et al. 1986; Milliganand Wood 1987). Physicalperturbations(e.g., tail grabbing) increase adrenaline levels to as high as 1 glmol L-' (Nakano L This content downloaded from 206.87.119.142 on Wed, 19 Nov 2014 15:54:21 PM All use subject to JSTOR Terms and Conditions 40 M.S. Graham andA.P.Farrell and Tomlinson 1967; Butler et al. 1986). Adrenalinelevels of 1 jLmol- L-1 produced maximalstimulationof perfused troutheartsat 10 C (Farrellet al. 1986). We comparedcardiacfunction with and without adrenergicstimulation to provide informationboth on the importanceof tonic adrenergicstimulation by the catecholamines normally found in the blood of resting fish and on the role of elevated blood catecholamines in stressed trout. An additional effect of temperatureis to significantlychange the blood viscosity of fish (Grahamand Fletcher 1984). Viscositydirectlyaffectsvascular resistance and therefore the amount of work performed by the heart to pump blood (Farrell 1984). This problem is compounded by the direct effect of temperatureon cardiacinotropy.Relativeheartweight increases in cold-acclimated trout (Farrell 1987; Farrell,Johansen, and Graham1988), goldfish (Tsukuda, Liu, and Fujii 1986), carp (Goolish 1987), and catfish (J. D. Kentand C. L. Prosser,personal communication). Thus, the increase in ventricle muscle mass could compensate for reduced inotropy and increased blood viscosity.We tested this hypothesis here. A working perfused heart was used to separate the direct and indirect effects of temperatureon the overall pumping ability of the heart (Graham and Farrell1985; Farrellet al. 1986). An advantageoffered by this approach is that chronotropic effects (intrinsic heart rhythm) and inotropic effects (maximumstrokevolume and pressuredevelopment) can be assessed with the same heartpreparation.The present studyused troutacclimatedto 5 and 15 C, and their in situ cardiac performancewas assessed as a function of acclimation temperatureand adrenergic stimulation. Chronic Q10values were derived for comparisons. andMethods Material Animals Rainbowtrout (Salmo gairdneri) were purchasedfroma local fishfarmhaving water temperaturesof 7-10 C year round. The fish were acclimated for at least 4 wk in 2,000-Ltankssupplied with flowing, dechlorinatedtapwater. The mean acclimation temperatureduring the winter months was 5.5 C (SEM = 0.1 C); fish acclimated to this temperaturewere used for experiments at 5 C. Meanacclimationtemperatureduringthe summermonthswas 15.5 C (SEM = 1.9 C); fish acclimated to this temperaturewere used for experiments at 15 C. The light-darkcycle for each time of year was maintained according to informationfrom the VancouverInternationalAirport This content downloaded from 206.87.119.142 on Wed, 19 Nov 2014 15:54:21 PM All use subject to JSTOR Terms and Conditions intheTrout Acclimation Heart41 Temperature (49"N latitude). Fish were fed commercial Fish Chow ad lib. five times per week. Pertinentmorphometricdataare found in table 1. Heart Preparation The procedurefor the in situ trout-heartpreparationfollowed thatdescribed elsewhere (Farrellet al. 1986), except thatthe temperatureof the perfusate going to the heart and the water for irrigatingthe gills approximatedthe experimental temperature.Preliminaryexperiments indicated that this approach significantlyreduced the experimental equilibration time. During surgerythere was minimal interruptionof flow to the heart and no direct physical manipulationof the heart.The input cannulato the heartwas introduced into the sinus venosus through a hepatic vein, and saline perfusion was begun immediately. Silk thread was used to secure the input cannula and to occlude the remaininghepatic veins. Separatesilk ligatureswere tied tightly around each ductus Cuvierto occlude these veins and to crush the cardiacbranchesof the vagus nerve. Smallerveins to the sinus venosus were not individuallytied off, but backflowinto small vessels was negligible (Farrell et al. 1986). The output cannulawas secured in the ventralaortavia an incision in the ventralbody wall. Preparationtime was 10-15 min. Forthe experiment the fish was fully immersed in a pH-adjusted(pH 7.9) Cortlandsaline baththatwas constantlyaerated.The input cannulareceived perfusate from a constant-pressurereservoir that was water jacketed. The output cannulawas connected to a pressurehead, and an in-line flow probe was placed in the output tubing near to the cannula.The input and output pressureswere measuredthrough saline-filled sidearmsconnected to pressure transducers.The perfusate going to the heart contained the following per liter: CaC12- 2H20 0.37 g, NaCl 7.25 g, KCl 0.23 g, dextrose 1 g, MgSO4 - 7H20 0.23 g, NaH2PO4 - H20 0.014 g, and Na2HPO40.33 g. The perfusatewas equilibratedwith a 0.5%/99.5%CO2/airmixture (PacificMedigas Ltd., Vancouver), and pH was brought to 7.9 after the addition of NaHCO3(1 g - L-'). The temperaturesof both the perfusateand the experimental chamberwere controlled at 5 C or 15 C with a thermostatedwater bath. Eachheartwas tested at the acclimationtemperatureonly. Heart rate in the in situ preparation was set by the intrinsic pacemaker rhythm (Farrell et al. 1986) and did not normally vary significantly under control conditions. Consequently, cardiac output (Q) was varied by altering stroke volume of the heart (SVH). SVHwas easily controlled by raising or lowering the height of the input-pressure head. The diastolic output pressure was varied by adjusting the height of the output-pressure head. This content downloaded from 206.87.119.142 on Wed, 19 Nov 2014 15:54:21 PM All use subject to JSTOR Terms and Conditions 42 M.S. Graham andA.P.Farrell 701 Fig. 1. An example of data recorded during a cardiovascular work challenge. Stable control conditions were establishedprior to the flow challenge. For the flow challenge, the input- Output Pressure cmH20O50 Input Pressure 05-, cmH2O 1 min Cardiac 20 Output mL min-l kg-1 pressure reservoir was raised while the outputpressure head was unchanged. Raising the inputpressure increased stroke volume and thus cardiac output. Inputpressure was raised until there was no further increase in stroke volume, and the associated cardiac output was termed "maximum cardiac output. " The change in inputpressure had no significant effect on heart rate. Inputpressure was lowered to restore the control cardiac outputprior to the pressure challenge. For the pressure challenge, the output-pressure head was first lowered and then raised in a stepwisefashion. Since inputpressure and heart rate were constant during the pressure challenge, any measured changes in cardiac output were a result of the change in outputpressure. Typically, lowering the outputpressureproduced a modest increase in cardiac output, while raising outputpressure compromised cardiac output. Excessive outputpressures could stop cardiac output entirely (table 1). o- IFlow Challengef I Pressure Challenge Experimental Protocols ControlCardiac Performance.Aftercompleting the surgery,each heartwas allowed to equilibrateto the experimentaltemperaturefor 5-20 min while it performed a control level of cardiacperformance.Stable heart rate (fH) and temperaturemeasurementsnearthe heartwere used to establish equilibration. Control Q was set at 10 mL - min-'1 kg-' at 5 C and at 20 mL min-'1 kg-1 at 15 C. Restingcardiacoutput in troutis 17 mL- min-' - kg-1L at 11 C (KiceniukandJones 1977). Controlmean outputpressurewas set at 50 cm H20 independent of temperature.Ventralaortic blood pressure in resting troutis 47-54 cm H20 (KiceniukandJones 1977). Cardiac WorkChallenge. To profile maximum cardiacperformance,each heart was presented with the same experimental work challenge. Cardiac work was increased in two ways: first,by increasing SVHto a maximum in orderto increaseflowwork,and, second, by raisingthe diastolic outputpressure to increase pressure work (fig. 1). The work challenge took approxi- This content downloaded from 206.87.119.142 on Wed, 19 Nov 2014 15:54:21 PM All use subject to JSTOR Terms and Conditions Acclimation intheTrout Heart43 Temperature TABLE 2 Effectof increasing outputpressure on theperfused heart at 5 C (N = 11) OutputPressure Adreneline Concentration 73 cm H20 85 cm H20 Adrenalinefree 1 nmol - L-1. 10 nmol . L-1............ 100 nmol - L-1 1 mol. L-1.......... 7 8 9 10 11 1 3 9 8 10 Note.Eachheartwasbrieflyexposedto eachpressure.Thenumberof preparations ableto concentration. generateflowat73 and85 cmH20is indicatedasa functionof adrenaline mately 10 min to complete. The control level of cardiacperformancewas restored before each subsequent experimental perturbation,and a further 5-min equilibrationwas allowed before the work challenge was repeated. Withthe diastolic output pressure constant,input pressurewas increased at a rate of 0.04-0.14 cm H20 - s-1 over 30-60 s until SVHdid not increase further.This was termed maximum SVH,and the associated Q was termed maximum Q. Control Q was restored after a stable level of maximum Q was recorded. Positive inotropic effects were indicated by an increase in maximum Q and/or a lower input pressure to generate the maximum Q (i.e., an increasedsensitivityto filling pressure). The relative stability of control Q as a function of output pressure was also used as a measure of inotropic performance.Since increasing output pressure ultimately compromised Q, positive inotropy was indicated by maintenance of control Q at a higher output pressure. To test this, input pressure was set to produce control Q, and mean output pressure was first lowered to 35-40 cm H20 and then increased in a stepwise fashion to 7375 cm H20 without changing input pressure. Outputpressurewas variedby adjustingthe height of the output-pressurehead. Qwas monitored throughout. All preparationscould generate an outflowat outputpressuresof 73-75 cm H20, but only some could generate an outflowat higher pressures (table 2). Therefore,a pressureof -73-75 cm H20 was adopted as a point of comparisonfor maximumpressuredevelopment. Effectof Adrenaline. Adrenergic effects were studied at 5 C and 15 C by This content downloaded from 206.87.119.142 on Wed, 19 Nov 2014 15:54:21 PM All use subject to JSTOR Terms and Conditions 44 M.S. Graham andA.P.Farrell using two experimental series. Adrenaline (=epinephrine HCl, Sigma, St. Louis) was used in all experiments. Freshadrenalinewas added to the perfusate just before the startof each test. Photodegradationof adrenalinewas limited by covering the perfusatecontainerswith foil. Experimentalseries I comparedmaximumcardiacperformancewith and without adrenaline in the perfusate (up to 1 gmol adrenaline - L-'). By the time fHhad stabilized in the experimental chamber, the hearts had been perfused with adrenaline-freesaline for at least 30 min (including surgery time). Therefore, it was assumed that the cardiacperformancemeasuredat this time had minimal adrenergic influence. Cardiacperformancewas first measured with adrenaline-freeperfusion by using the work challenge and then was reexamined for a cumulativelog concentrationrangeof adrenaline (1 nmol - L-', 10 nmol . L-', 100 nmol - L-, and 1 gmol - L-'). The heart was allowed to equilibratefor 5 min at each adrenalineconcentrationbefore performingthe work challenges. These experiments lasted --100 min. Experimental series II compared maximum cardiac performance with adrenaline concentrations of 5 nmol - L-1, 10 nmol . L-', and 50 nmol -' in a manneridentical to thatof series I, except thatthere was no adrenalinefree perfusion. The heart received perfusate containing 5 nmol adrenaline - L-1 during surgery.This initial adrenaline concentrationwas established in partbecause adrenaline-freeperfusion at 5 C in series I produced slow and irregularrhythms (no beats for up to 4 s) and an unusually poor response to filling pressurein manypreparations,which were consequently discarded. (Irregularheartbeatswere rare at 15 C in series I.) Preliminary experiments indicated thatthe presence of 5 nmol adrenaline - L-1(but not of 1 nmol adrenaline - L-') in the initial perfusateprevented these arrhythmias at 5 C. The experiments in series II lasted --60 min. Since an adrenalineconcentrationof 5 nmol . L-' is similarto thatfound in resting trout,comparisonsof cardiacperformanceat 5 nmol adrenaline L-1'in series II with adrenaline-freeperfusion in series I provided a means to evaluate the role of tonic adrenergic stimulation of the heart by bloodborne catecholamines. Furthermore,since the maximum adrenaline concentrationused in series II (50 nmol - L-1)is similarto the elevated plasma levels observed after stressful exercise in trout, comparisons can be made with series I, where there was maximalstimulationof the heartwith 1 p1mol adrenaline . L-7. Time Trials.The time-trialexperimentswere designed to assess anydeterioration of cardiacperformancewith time. The protocol was similar to that used in series I in thatthe work challenge was repeated five times consecu- This content downloaded from 206.87.119.142 on Wed, 19 Nov 2014 15:54:21 PM All use subject to JSTOR Terms and Conditions intheTrout Acclimation Heart45 Temperature tively but with no adrenaline present. The time trials could only be performed at 15 C because prolonged exposure to adrenaline-freeperfusion at 5 C resulted in cardiac arrhythmias.These experiments typically lasted 80 min. Measurementsand Calculations The input pressureto the sinus venosus and the output pressure in the ventralaorta,immediatelyanteriorto the bulbus arteriosus,were measuredcontinuously. Pressuresignals (LDI-5;Narco Telecare, Houston) were amplified appropriatelybefore being displayed on a chartrecorder (Gould 2400; Gould, Ohio). The resistancesof the output and input cannulaewere determined with known flow rates of perfusate,and all pressure measurements were corrected accordingly. Outflow was measured continuously with an in-line electromagnetic flow probe (SWF-4;Zepada Instruments,Seattle) placed in the outputtubing immediatelyafterthe outputcannula.Meanflow values were recorded. The flow probe was calibratedwith known flow rates of perfusate.Representative10-s samples of the analogue pressureand flow signals were converted to digital signals and stored on computer disk for subsequent analysis (Farrell and Bruce 1987). Cardiacoutput was determined as the productof SVHand fHand was expressed in mL - min-' - kg-1 (where kg refers to the total wet mass of the fish). Mass-specificpower output of the heartwas calculated as (Q X [outputpressure - input pressure] X 0.00163)/g and was in units of mW/g (where g refersto the totalwet mass of the ventricle). To assess the importanceof ventricle size on cardiacpower output, absolute power output and absolute stroke work were also calculated. Absolutepower output (mW) = (mass-specificpower output) X (ventricle mass), and absolute stroke work (mJ) = (absolute power output)/ (heartrate/60). StatisticalProcedures Repeated-measuresanalysis of variancewas used to compare mean values. Unpairedt-testswere used to compare mean values between temperatures. Statisticalprocedures were performed using the packages available on the IBMmainframecomputerat Simon FraserUniversity.Significantdifferences were at the 95%confidence level. This content downloaded from 206.87.119.142 on Wed, 19 Nov 2014 15:54:21 PM All use subject to JSTOR Terms and Conditions 46 M.S. Graham andA.P.Farrell Results Time Trials The cardiovascularvariablesassociatedwith control and maximumQ conditions are presented in table 3 for each of the five consecutive work challenges, the entire series lasting --80 min. In the firsttrial with adrenalinefree perfusion,raisinginputpressureby 2.5 cm H20 approximatelydoubled SVH, Q, and power output without a significantchange in fH;fH decreased with subsequent adrenaline-freeperfusion such that, in the second trial, control fHwas reduced by 14%,and, in the thirdtrial,control fHwas reduced by a further4%.ControlfHwas unchanged duringthe fourthand fifthtrials. The significantdecrease in fHbetween the firstand second trials required that, in order to maintain control Q, input pressure be raised to increase control SVH. MaximumSVH,Q, and power output were not significantlydifferentbetween the firstand second trials.There was a trendtowarda lower maximum SVH,a result that, coupled with the trend towarda higher input pressure to stimulatemaximumSVH,suggests thatthere was a minor inotropic deteriorationby the fifthtrial.The net effect of this chronotropicand inotropicdeteriorationwas that maximumQ and power output were reduced by 10%for the second trial and by 16%,19%,and 21%for the third, fourth, and fifth trials, respectively. The initial decrease in fHwas the majorreason for the changes. The time-dependent change in fHwas importantin interpreting datain series I. Series I ControlConditions.Withthe adrenaline-freeperfusion (table 4), the intrinsic fHwas significantlyhigherat 15 C thanat 5 C. Thus,control SVHwas made similarat both experimentaltemperaturesso thatthe control Q at 15 C was set to twice that at 5 C. A similar input pressure was used at both temperatures to produce the control SVH. Adrenalineproducedpositive chronotropiceffectsat 5 C andat 15 C (table 4). Comparedwith adrenaline-freeperfusion, 1 jimol adrenaline . L-1produced a significant increase in fH at both experimental temperatures (14.4 beats . min-1 at 5 C and 11.6 beats . min-1 at 15 C). In addition, comparison of fHfor the time trials (table 3) and series I (table 4) indicates that a concentration of adrenaline >1 nmol L-1 offset the initial chronotropic deterioration seen with adrenaline-free perfusion in the time trials. If the lower concentrations of adrenaline had not affected fH, there should have been a sig- This content downloaded from 206.87.119.142 on Wed, 19 Nov 2014 15:54:21 PM All use subject to JSTOR Terms and Conditions letter g-1) (.40)4.07b (.72) (.48)3.90c (.63) 5.02abc Maximum 4.52(.41)4.22a (mW. superscript Power Control 2.50(.30) 2.63(.30)2.44(.31)2.57(.23)2.82(.38) same the kg-1) having . (3.93) (2.68) (2.99) (3.96) Maximum 34.6b 42.4abc 38.6(3.69) 35.8a 32.9c min-1 - column each Q (mL Control20.2(.62)21.2(.63)19.6(.95)21.1(1.02) 23.1(1.68) within Values kg-1) Maximum .69 (.089) .63 (.073) .70 (.080) .68 (.071) .62 (.074) min. 15 (mL about 39a(.037) .32abcd (.028) .39C (.021) .37b(.032) SVH Control .43d(.032) experiments trial min-1)Maximum (5.1) (4.3) (3.9)55.7c 53.6b (3.3) (2.6) 63.1abcd 56.2a 53.5d time-trial the in (beats. fH (5.1) (4.8) (4.0)53.8c Control (4.1) (4.5) 56.2a 54.0b 53.8d 64.2abcd (SEM). means Maximum 2.57(.62) 2.46(.65) 2.46(.52)2.51(.35)3.03(.50) represent Control.11 (.24).10 (.21).12 (.19).31 (.20) .68 (.60) and C 15 for different are cardiacPressure H20) (cm Input maximum and 1 Control TABLE Each 4. N= output 3 lasted 2 3 4 5 Trial Trial Trial Trial Trial This content downloaded from 206.87.119.142 on Wed, 19 Nov 2014 15:54:21 PM All use subject to JSTOR Terms and Conditions values Allsignificantly 0.05). (P< Note. were C 15 (.098) (.11)2.04* (.54) (.12) (.098) 2.10* 2.04* 2.07* 2.06* marked g-1) C (mW. 5 Power .87 (.031) .84 (.050) .80 (.049) .78 (.062) .82 (.054) between adrenaline * kg-') - C 15 (.54)19.47* (.58)19.10* (.50)19.35 (.68)19.15* (.36) 19.46* 0.05) each < (P within 9.87(.41) 9.61(.49)10.13 (.31)10.84 (.27) (.34)10.35 groups differences min-1 C Q (mL 5 C kg-') 15 . .29a(.015) .37 (.033) .35 (.029) .39 (.029) .35a(.018) C SVH 5 .27a(.011) .33(.026) .44 (.044) .48 (.058) .43a(.042) C 15 (3.07) (4.36) (3.84) (3.02) (3.73) 53.6* 57.1* 68.7d,* 57.12*a 50.8* min-1) - and C 5 at C fH (beats 5 C 15 Pressure H20) experiments I C (cm 5 Input and C,indicates (.076) 5 .040',* .16 (.12) .42a(.21).23 (.12).21 (.14) for 11 asterisk N= .46 (.11).31a(.096) .54a(.12) .66 (.15).43 (.12) for free values L-1 L-1 . L-1 L-'...... nmol nmol 100 1 Concentration Adrenaline 10 Adrenaline (SEM). superscript A means letter. are same Values the nmol Control TABLE 0.05) < (P superscripts Lettered difference C. 15 for (1.02) 7 significant (3.11) 25.8(2.93) 33.3(2.29) 23.1(3.25) 40.3a 25.9a a N= Series 4 significant temperature indicate between (mL C 15 trial. values jmol 1 This content downloaded from 206.87.119.142 on Wed, 19 Nov 2014 15:54:21 PM All use subject to JSTOR Terms and Conditions Note. with intheTrout Acclimation Heart 49 Temperature nificantdecrease in fH,similarto thatseen with adrenaline-freeperfusion in the time trials.This was not the case. With 10 nmol adrenaline - L-1,fHwas the same as the initial condition at 5 C and was only 6%lower at 15 C (table 4). By comparison,fHwas reduced by 18%during the third time trial with adrenaline-freeperfusion (table 3). Because 1 pmol adrenaline - L-1produced a tachycardia,input pressure was lowered to significantlyreduce control SVuand to set the control Q. Althoughcontrol SVHwith 1 pmol adrenaline - L-1was comparableat both experimental temperatures,input pressure was significantlylower at 15 C comparedwith 5 C (table 4). There was no significantdifference between input pressuresat 5 C and at 15 C for other adrenalineconcentrationsor for adrenaline-freeperfusion. This indicates that the perfused trout heartwas more sensitive to filling pressureat 15 C in the presence of high adrenaline concentrations. Flowand PressureChallenges.Forthe 5 C and 15 C experiments,the cardiovasculardata for maximum Q conditions at various adrenaline concentrations are presented in table 5. Withadrenaline-freeperfusion, raising input pressureby 3 cm H20 produced a maximumQ thatwas approximatelytwice the control Q. Comparedwith adrenaline-freeperfusion, maximumQ with 1 jmol adrenaline - L-' was increased by 62%at 5 C and by 25%at 15 C. There was a significantadrenergicstimulation of fHand maximumSVHat 5 C but a significantincrease only in fHat 15 C (table 5). Even though maximum SVHwas unchangedat 15 C with adrenergicstimulation,1 pmol adrenaline . L-' increased the sensitivity of the heart to input pressure, as indicated by a significantlylower input pressure associated with maximumSVH (table 5). The pressurework challenge revealed that 1 pmol adrenaline . L-' had a positive inotropic effect at both experimental temperatures.With adrenaline-free perfusion, raising the output pressure above 70 cm H20 reduced Q by 17%at both experimental temperatures(figs. 2A, 2B). At 5 C, 1 .tmol adrenaline - L-' completely prevented this decrease in Q (fig. 2A) and also permitted flow at output pressures up to 85 cm H20 (table 2). At 15 C, the inotropic effect of 1 pmol adrenaline L-1was effective at maintainingQ at elevated output pressures, although it was not as effective at doing so as it was at 5 C. Series II Control Comparisonsbetween series I and series II clearly demonstrated the importanceof tonic adrenergicstimulationwith an adrenalineconcen- This content downloaded from 206.87.119.142 on Wed, 19 Nov 2014 15:54:21 PM All use subject to JSTOR Terms and Conditions C 15 (.25) (.25)3.49* (.26)4.02* (.31)4.93a* (.31) 3.90a* 3.62* C (mW. 5 Power (.16)1.71(.16)1.93(.19)2.50(.15)2.88a 1.76a (.10) g-1) * experiments I min-1- C 15 (1.97) (2.29) (2.39) (3.22) (3.16) 39.50* 34.33* 38.38a,* 47.23a,* 35.73 table in as - Series C Q (mLkg-1) 5 Cfor 15 4. (1.80) (1.62) (2.06) (1.56) (1.40) 22.06 24.98 31.12a 35.98b 22.30ab indicated C kg-') 15 and C 5 at are .71 (.055) .74 (.044) .70 (.033) .69 (.035) .72 (.032) 0.05) (P< (mL C SVH 5 (.031) .92d(.037) .90b(.034) .95c(.034) .81a(.042) .75abcd differences conditions flow C 15 min-') (2.56) Significant (2.74) (3.86) (4.24) 54.2* 53.9a.* 51.4(3.54) 50.1* 67.7a'* C. 15 C fH (beats 5 maximum C 15 during * (1.20) (2.31) 28.0(2.31) 32.9(1.66) 39.3a 30.0a 27.7(2.19) N= (.38) 2.26* 3.53(.66)3.49(.50)3.13(.43)3.10(.61) and C, 5 for 11 H20) C (cm 5 Input Pressure for 7 3.57(.34)3.75(.28)4.18(.29)3.09(.25)3.28(.28) N= (SEM). valuesproduced free 5 L-1 - L-l - L-1 - means L-1 are - nmol nmol Mmol nmol 100 1 1 10 Cardiovascular Adrenaline Concentration TABLE Adrenaline This content downloaded from 206.87.119.142 on Wed, 19 Nov 2014 15:54:21 PM All use subject to JSTOR Terms and Conditions Values Note. Acclimation intheTrout Heart51 Temperature A 2.0 30 C 2.0- 0 5030 70 -2.0 70 -2.0- 03 2.0- 2.00 30 70 70 So I -4.0- ,~ -2.0 -2.0- Seriesll- 50C N-6 -4.0- Output Pressure, SeriesTl-15C N.9 cmH20 Fig. 2. Thepressure challenge produced changes in the resting cardiac output (Q). The change in resting Q (AQ) ispresented as afunction of the outputpressure for the various adrenaline concentrations tested in series I and series II. Symbols represent thefollowing adrenaline concentrations: series I, O = 1 mol - L-', 9 = 100 nmol L- A = 10 nmol L-', E = 1 nmol L-, 0 = adrenaline-free; series II, A = 50 nmol . L-J, A = 10 nmol - L-', * = 5 nmol - L-1. For series I:panelA, N = 11 (5 C);panel B, C, N = 7 (15 C). For series II:panel C, B, N = 6 (5 C); panel D, N = 9 (15 C). Allpoints are means, and vertical bars represent SEM. trationsimilar to that found in the plasma of resting trout. Initial perfusion with 5 nmol adrenaline - L-1in series II completely prevented the arrhythmicity and time-dependent decrease in fHthatwere associatedwith adrenaline-free perfusion at 5 C in series I. As in series I, fHin series II was significantlygreaterat 15 C than at 5 C at all adrenalineconcentrations(table 6). At 5 C the initialfHat 5 nmol adrenaline - L-1 (table 6) was significantlygreaterthan that with adrenaline-free This content downloaded from 206.87.119.142 on Wed, 19 Nov 2014 15:54:21 PM All use subject to JSTOR Terms and Conditions C 15 2.16(.11) 2.16(.12)2.14(.08) 3.80(.18) (.18) (.22) 4.08b 4.58b g-l) C (mW. 5 Power .87 .81 .83 (.070) (.063) (.070) 2.38(.19)2.38(.19)2.58(.17) output cardiac of level the to kg-1') C 15 (.54) (.60) (.29) 20.14*20.06* 20.22 (2.10) (2.86) refer (2.04) 35.56* 39.39b,* 44.58b,* min-1' C 15 C Q (mL 5 and C 5 at II) C kg-1) 15 . "maximum" (.38) (.16) (.38) 10.64 9.98 10.17 (2.87) (2.89) (3.03) 30.42 31.00 33.17 and .43 (.032) .41a(.025) .37a(.014) .77(.035) .81 (.035) .82 (.036) "Control" (mL C (Series SVH 5 C 15 min-1) adrenaline of C fH (beats. 5 levels C 15 Pressure H20) tophysiological C (cm 5 Input .30 (.031) .30 (.036) .26 (.030) .83 (.074) .82 (.056) .85 (.059) experiments. C 4. 15 * fortable a* 9 in as (3.0) (1.7) 48.4(3.0) (1.6)54.4b,* (1.6) N= 48.5* 49.8(2.1)55.8a'* 48.9b,* 36.7(3.1)35.5(3.3)40.4(3.1) 37.2(2.7) 36.8(1.9)39.2(2.5) * .31 .19* .18* (.12) (.10) (.14) 2.33(.61) (.35)2.13* (.27) 2.46* . .68 .74 .70 (.21) (.16) (.13) 3.23(.25) 3.96(.49)3.29(.28) and indicated are 0.05) experiments, C 5 (P< for 6 N= differences (SEM). response L-1 L-1 - L-1 L-1 - L-1 L-1 . 6 nmol nmol nmol nmol nmol nmol 10 10 5 5 50 50 Cardiovascular Concentration Control: TABLE Maximum: Adrenaline This content downloaded from 206.87.119.142 on Wed, 19 Nov 2014 15:54:21 PM All use subject to JSTOR Terms and Conditions Significant means are values experiment. All each Note. in Acclimation intheTrout Heart53 Temperature perfusion in series I (table 4). In addition, the fHat 50 nmol adrenaline L-' in series II was not significantlydifferentfrom the fHat 1 Ilmol adrenaline - L-1in series I. This comparisonemphasizes the importanceof tonic adrenergicstimulationof fHat 5 C. Comparedwith the 5-nmol - L- adrenaline concentration, both the 10- and 50-nmol - L-1adrenaline concentrations significantlyincreased fHat 15 C but not at 5 C (table 6). Flow and Pressure Challenge. Raising input pressure had no significant effect on fHat either experimental temperature(table 6). MaximumQ was significantlygreaterat 15 C thanat 5 C, which reflecteda significantlyhigher fH at 15 C (table 6). Comparedwith the 5-nmol - L-' adrenaline concentration, both the 10- and 50-nmol - L-Uadrenaline concentrations increased maximum Q significantlyat 15 C but not 5 C. Comparedwith the 100- and 1-pmol - L-1adrenaline concentrationsin series I (table 5), the 50-nmol L-' adrenaline concentration in series II (table 6) did not show a significantlydifferentmaximumQat either experimentaltemperature. The positive inotropic effect of adrenalinewas qualitativelyand quantitatively similar to that in series I. Adrenergicstimulationincreased the sensitivity of the heart to filling pressure at 15 C but not at 5 C, since the input pressure required to generate control SVHand maximum SVHwas significantly lower at 15 C than at 5 C (table 6). Furthermore,when the output pressurewas increasedto - 70 cm H20, 50 nmol adrenaline L-1prevented a significantdecrease in Q at 5 C (fig. 2C); at 15 C 50 nmol adrenaline - L-I partiallyoffset the decrease in Q (fig. 2D). Chronic Q1c Values. The positive chronotropic and inotropic effects of adrenaline were qualitativelysimilar for perfused hearts from trout acclimated to 5 C and 15 C. However, there were quantitativedifferences,which were apparentwhen Qiovalues were compared. The QO0for fHwas 2.20 with adrenaline-freeperfusion; 1 jtmol adrenaline - L-1 reduced this Qo0to 1.70 in series I, and in series II the Q10for fH was 1.38 with 50 nmol adrenaline - L-'. Adrenergic stimulation therefore clearly compensated for the direct effect of temperatureon the intrinsicfH,. This compensation was also reflected in the maximumQ.The Qio for maximum Q was 1.72 with adrenaline-freeperfusion; 1 jimol adrenaline L-I reduced this Q10to 1.31 in series I, and in series II the Q10was 1.34 at 50 nmol adrenaline L-1. Heart Size. Heart mass was significantly larger in cold-acclimated trout (table 1). Relative ventricle mass (expressed as a percentage of body mass) This content downloaded from 206.87.119.142 on Wed, 19 Nov 2014 15:54:21 PM All use subject to JSTOR Terms and Conditions 54 M.S. Graham andA.P.Farrell was --50% greaterin 5 C-acclimatedtrout.The importanceof this increase in ventricle mass on cardiac performancewas seen in two ways: first, by comparing the maximum values for absolute power output and mass-specific power output and, second, by comparing absolute stroke work of the heartat the two experimentaltemperatures. The Q10of 1.78 for the maximum value of mass-specificpower output indicated that there was little temperaturecompensation per gram of muscle. However,the Qo0for absolute power outputwas 1.34 and indicatedthat the increase in ventricle mass provides partialcompensation for the direct effect of temperatureon inotropy.A similar conclusion was reached when absolute strokeworkwas calculated.Maximumstrokeworkwas consistently greaterin cold-acclimatedhearts (rangingfrom 2.25 mJ to 2.81 mJ) than in warm-acclimatedhearts (rangingfrom 1.12 mJto 2.12 mJ) (calculatedfrom datain tables 1, 5, 6). Thus, the work per beat of the relativelylargerhearts in cold-acclimated trout can exceed that in the hearts of warm-acclimated trout,although the warm-acclimatedtroutheartcan beat faster. Discussion Adrenergic Stimulation In these experiments we studied the effects of adrenaline, even though adrenaline and noradrenalineare found in similar concentrations in the blood and heart tissue/nerve endings at rest (Abrahamssonand Nilsson 1978; Pennec and LeBras1984). The selection of adrenalineas the sole adrenergic agonist was based on the fact thatadrenalineis generally 10 times more effective than noradrenaline in stimulating P-adrenoceptorsin the troutheart (Ask, Stene-Larsen,and Helle 1981; Farrellet al. 1986). Furthermore, following stressful exercise, adrenaline is the dominant hormone in trout (Nilsson 1983), although noradrenalineis the dominant neurotransmitterreleased into perfusatefollowing vagal stimulationof perfused goldfish hearts(Cameronand O'Connor1979). The present study demonstratedin several ways that the resting level of circulatingcatecholamines (1-9 nmol - L-1;Woodward1982;Axelsson and Nilsson 1986; Primmettet al. 1986; Milligan and Wood 1987) provides an important, if not essential, cardiac tonus in trout. First, the time-trial experiments at 15 C showed initial chronotropic and then progressive inotropic deterioration with adrenaline-free perfusion. Second, preparations were discarded because they became arrhythmic and unresponsive to filling pressure at 5 C with adrenaline-free perfusion. Even with hearts that were relatively This content downloaded from 206.87.119.142 on Wed, 19 Nov 2014 15:54:21 PM All use subject to JSTOR Terms and Conditions intheTrout Heart55 Acclimation Temperature stable at 5 C, adrenaline-freeperfusion could not be prolonged much beyond 30 min without deterioration.Third,in series II, initial perfusionwith 5 nmol adrenaline - L-1prevented these chronotropicand inotropic problems at 5 C. The importanceof adrenalinefor successful perfusion of isolated and in situ trout hearts has been noted elsewhere (Bennion 1968; Farrellet al. 1986). There are several indications that the tonic effect of adrenaline at colder temperaturesmay be particularlyimportantin stimulatingthe sinoatrialpacemakerand in preventingatrioventriculardesynchronization.Bennion (1968) used 300 nmol adrenaline - L-1to preventthe weak contraction and atrioventricularblock associatedwith adrenaline-freeperfusion,but she made no distinctionbetween the adrenergiceffect at 6 C and at 15 C. Farrell et al. (1986) found that only four of 75 in situ heart preparationsshowed serious arrhythmiasat 10 C with initial adrenaline-free perfusion; subsequent perfusion with >10 nmol adrenaline - L-1prevented arrhythmia.In the present study, arrhythmiawas frequent at 5 C but was absent at 15 C. Adrenergiceffects on atrioventricularconduction were also reportedat 8 C for the eel (Anguilla anguilla). In the eel, a-adrenoceptorswere stimulated at adrenaline concentrations>5 jimol - L-1to produce desynchronization (Pennec and Peyraud1983). However, the adrenergiceffects in the eel are clearly the opposite of those found in the trout both in terms of the effect and in terms of the type of adrenoceptor involved. (Positive inotropy and chronotropyare mediated by P-adrenoceptors[Asket al. 1981;Cameronand Brown 1981; Farrellet al. 1986; Temma et al. 1986] without involvement of a-adrenoceptorsin trout [Salmogairdneri], goldfish [Carassiusauratus], carp [Cyprinuscarpio], and flounder [Pleuronectesplatessa] but not perch [Percafluviatilus][Tirriand Lehto 1984].) The present study also found that the progressive inotropic deterioration associated with adrenaline-freeperfusion was ameliorated by adrenaline. This phenomenon may be related to-but not necessarily limited to-the absence of adrenergicstimulationof metabolism, adrenergicstimulationof transsarcolemmalcalcium movement, or progressive atrialoverdistension. Atrialoverdistension was observed in isolated trout hearts during adrenaline-free perfusion (A. P. Farrell,unpublished observation)and was amelioratedby adrenaline.However,atrialoverdistension may not be a concern in intacttrout,in which the atriumis constrainedwithin the pericardium(Farrell et al. 1988). Although the present study established the importanceof tonic humoral stimulationof the heart under resting conditions, there is normallya complex interplaybetween excitatoryadrenergictonus and inhibitorycholiner- This content downloaded from 206.87.119.142 on Wed, 19 Nov 2014 15:54:21 PM All use subject to JSTOR Terms and Conditions andA.P.Farrell 56 M.S. Graham gic (vagal) tonus in intact teleosts under resting conditions (Axelsson, Ehrenstrom,and Nilsson 1987). Adrenergicstimulation of the fish heart is possible throughthree mechanisms:circulatingcatecholamines,adrenergic innervation,and cells containingcatecholamines.Adrenergicnerves,which enter the sinus venosus through cardiacbranches of the vagus nerve, converge on the sinoatrialplexus (pacemaker) and to some extent along the atrialcanaland the atrioventricularfunnel (Laurent,Holmgren,and Nilsson 1983). Also, adrenergicinnervationis associated with the coronaryvasculature (Holmgren 1977) and so is more dense in the compact myocardium (Yamauchiand Burnstock1968). In addition to storage in nerve terminals, Yamauchiand Burnstock (1968) demonstrated the presence of catecholamines in granularvesicles in the sarcoplasmof the troutheart.Since nothing is known about the levels of catecholamines released from storage granules or nerve terminals, the results of the present study apply only to adrenergic stimulation of the heart through blood-borne catecholamines. The adrenaline concentrationsused here were within physiological limits, although the maximumlevel used in series I (1 pmol - L-) should be considered representativeonly of plasmalevels of troutundergoingsevere handling stress. Adrenaline levels similar to those associated with stressful exercise produced positive inotropic and chronotropic effects at 15 C (series II) that were comparable with those previously observed both at 10 C for in situ perfused hearts (Farrellet al. 1986) and at various temperaturesfor atrial strips (Asket al. 1981). At 5 C, inotropicand chronotropiceffects of adrenaline were limited to those produced by tonic stimulation. This finding is consistent with the previous observationthatadrenergicstimulationof fHis reduced in troutacclimatedto 5 C (Wood et al. 1979). In contrast,adrenergic stimulation of maximumtension was three times greaterat 2 C than at 14 C in atrialstrips taken from troutacclimatedto 8 C and tested at 2 C and at 14 C (Asket al. 1981). This greaterinotropiceffect of adrenalineat a lower temperaturecontrastswith the present results and may reflect a difference between an acute temperaturechange and temperatureacclimation. Temperature Effects The present study revealed direct and indirect effects of temperature on cardiac performance. Maximum Q was apparently affected more by temperature-dependent changes in fHthan it was by temperature-dependent effects on inotropy. An increase in heart mass with cold acclimation and differences This content downloaded from 206.87.119.142 on Wed, 19 Nov 2014 15:54:21 PM All use subject to JSTOR Terms and Conditions Acclimation intheTrout Heart57 Temperature in adrenergicstimulationpartiallycompensated for the direct effects of temperatureon the intrinsicmechanicalpropertiesof the troutheart. The direct effect of temperatureon fHhas been well documented by experiments involving acute temperaturechanges. In general, the acute Q10 for fHis --2.0 for isolated hearts and for intact fish. For goldfish hearts in vitro, the Q0ofor fHwas 2.0 and 1.6 for acclimation temperaturesof 25 and 10 C, respectively (Tsukudaet al. 1986). For isolated trout hearts, the Q10 for fHwas 2.4 (Bennion 1968). In perfused sea ravenhearts (Hemitripterus americanus), Q0ofor fHwas 1.9 and 1.4 for acclimation temperatures of 5 C and 15 C, respectively (Graham and Farrell 1985). The Q1ofor fHwas 1.76 for intact trout (Hughes and Roberts1970), 2.6 for intact carp (Moffittand Crawshaw1983), 2.1-2.5 for intact winter flounder (Pseudopleuronectes americanus) (Cech et al. 1976), and 1.78-2.78 for the intact eel (Seibert 1979). Thus, it appearsunlikely that there is little compensation of resting fH in intactfish duringan acute temperaturechange. In contrast,chronic temperaturechanges are accompanied by a compensation of resting fH in intact fish. The Q1ovalues for fH derived from intact fish acclimated to different temperatureswere generally <2.0 (1.5 for the trout[Priede1974],2.6 for the trout[Woodet al. 1979],1.2 for the eel [Seibert 1979], and 1.3-1.6 for winter flounder [Cech et al. 1976]). Most evidence suggests that this temperaturecompensation involves extrinsic modulation ratherthan the pacemakerper se. Forexample, the Q10for fHwas increased to 2.0 in intactfish afteradrenergicor cholinergic modulationof fHwas surgically or pharmacologicallyblocked (Priede 1974; Siebert 1979;Wood et al. 1979). Similarly,with adrenaline-freeperfusion in vitro, the Q0ofor fHwas 2.2 for the trout (present study), 2.0 for the sea raven (Grahamand Farrell 1985), and 1.7 for the eel (Tsukudaet al. 1986), and in the present study adrenergicstimulationsignificantlyreduced the Q0ofor fHfrom 2.20 to 1.38. Modulationof cholinergic inhibition of fHis also importantduringtemperature acclimation and has been considered elsewhere (Priede 1974; Siebert 1979;Wood et al. 1979). Although many studies have provided informationon how temperature acclimation affects fH, little is known concerning temperatureeffects on SVH.The present study is the firstto compare the regulationof SVHin coldand warm-acclimatedtrout. SVHis influenced by the volume of the heart chambers, filling pressure, filling time, and the inotropic state of the heart (Randall 1970; Farrell 1984). The cold-acclimated trout heart was generally less sensitive to filling pressure in the presence of adrenaline (tables 5, 6). This probably reflects a direct effect of temperature, since the perfused sea raven heart responded similarly to an acute, as well as to a chronic, tempera- This content downloaded from 206.87.119.142 on Wed, 19 Nov 2014 15:54:21 PM All use subject to JSTOR Terms and Conditions 58 M.S. Graham andA.P.Farrell ture change (Grahamand Farrell1985). Nevertheless, maximumSVHof the heartwas the same or greaterin cold-acclimatedcomparedwith warm-acclimated trout. This is an importantfinding because it implies that cole and warm-acclimatedtroutare equally capable of exploiting the maximumvolume of the heartchambers,provided thatthere is adequateadrenergicstimulation and thatthere is no limitationon venous returnpressure. Perhapsthe most importantcompensationfor the directeffect of temperature on inotropy was the --50% increase in relative ventricle mass; an increase in the number of contractileunits in the ventricle compensated for the relativelyweaker contractionof individualunits, as indicatedby the fact thatabsolute strokework was higher in cold-acclimatedthan in warm-acclimated trout hearts.The consequence of increasing the relative heart mass in cold-acclimatedtroutwas veryclear.The chronic Q1ofor maximumQ was -1.34 despite temperature-relateddifferences in fH.This Qo0representsa --66% compensation. An increase in relative heart mass during cold acclimation has been reported elsewhere for a variety of teleosts, including trout (Tsukudaet al. 1986; Farrell 1987; Goolish 1987; Farrellet al. 1988;J. D. Kent and C. L. Prosser, personal communication). While muscle protein increased with these increases in heart mass, cardiac growth in trout involves significant myocyte hyperplasiaas well as myocyte hypertrophy(Farrellet al. 1988). It is not clear at this time which of these two mechanisms operates in trout during temperatureacclimation. However, it does seem likely that an increase in heartmass may be a general mechanismfor temperatureconipensation among teleosts. The present observationsand conclusions regardingthe effectof temperature on SVHseem consistent with those of previous studies on intact fish. Winter flounder increase resting Q by increasing both SVHand fHduring temperatureacclimation (Cech et al. 1976), whereas increases in fHare the primarymeans of increasing resting Q during acute temperaturechanges (Stevens et al. 1972;Cech et al. 1976). In addition, Priede (1974) calculated that, during swimming, SVHincreased more than twofold in both 6 C- and 15 C-acclimated trout, which is consistent with our suggestion that maximum SVHis not compromised at low watertemperatures. In summary,the present study indicates that resting levels of circulating catecholamines probablyimpartan importantcardiactonus in intact trout. At 5 C this tonus appearedto be more importantin preservingcardiacrhythmicity, while at 15 C it stimulatedinotropyto a greaterdegree. There was a direct effect of temperatureon fH,which affectedmaximumQ and was partially compensated by tonic adrenergicstimulation.Because maximumSV, This content downloaded from 206.87.119.142 on Wed, 19 Nov 2014 15:54:21 PM All use subject to JSTOR Terms and Conditions intheTrout Acclimation Heart59 Temperature was unaffectedby temperature,there was a 66%compensation of maximum Q. Ventriculargrowth,stimulatedduringseasonal cold acclimation,contributed directly to maintainingmaximum SVHand stroke work in cold-acclimated trout.These compensations may be importantin maintaininga high level of cardiacperformance-and hence of swimming performance--during winter months. Acknowledgments JeffJohansen is thankedfor his technical assistance,especially with the statistical analysis. This study was funded by the NaturalSciences and Engineering Council of Canadathrough an operating grant to A. P. Farrelland by a postdoctoralfellowship to M. S. Graham. Literature Cited 1978. Control of catecholamine release from chroT., and S. NILSSON. ABRAHAMSSON, L. BOLIs,and maffin tissue in a teleost fish. Pages 247-252 in K. SCHMIDT-NIELSEN, S. MADDRELL, eds. Comparative physiology-water, ion and fluid mechanics. Cambridge University Press, Cambridge. ASK, J. A. 1983. Comparative aspects of adrenergic receptors in the hearts of lower vertebrates. Comp. Biochem. Physiol. 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