Literature DB >> 1522520

Changes of intracellular pH due to repetitive stimulation of single fibres from mouse skeletal muscle.

H Westerblad1, D G Allen.   

Abstract

1. The performance of skeletal muscle during repetitive stimulation may be limited by the development of an intracellular acidosis due to lactic acid accumulation. To study this, we have measured the intracellular pH (pHi) with the fluorescent indicator BCECF (2',7'-bis(carboxyethyl)-5(6)- carboxyfluorescein) during fatigue produced by repeated, short tetani in intact, single fibres isolated from the mouse flexor brevis muscle. 2. The pHi at rest was 7.33 +/- 0.02 (mean +/- S.E.M., n = 29, 22 degrees C). During fatiguing stimulation pHi initially went alkaline by about 0.03 units (maximum alkalinization after about ten tetani). Thereafter pHi declined slowly and at the end of fatiguing stimulation (tetanic tension reduced to 30% of the original; 0.3Po), pHi was only 0.063 +/- 0.011 units (n = 14) more acid than in control. 3. We considered three possible causes of acidosis being so small in fatigue: (i) a high oxidative capacity so that fatigue occurs without marked production of lactic acid; (ii) an effective transport of H+ or H+ equivalents out of the fibres; a high intracellular buffer power. 4. The oxidative metabolism was inhibited by 2 mM-cyanide in three fibres. After being exposed to cyanide for 5 min without stimulation, the tetanic tension was reduced to about 0.9 Po and pHi was alkaline by about 0.1 units. The fibres fatigued faster in cyanide and the pHi decline in fatigue was more than twice as large as that under control conditions. 5. Inhibition of Na(+)-H+ exchange with amiloride resulted in a slow acidification of rested fibres; resting pHi was not affected by either inhibition of HCO3(-)-Cl- exchange with DIDS (4,4'-diisothiocyanatostilbene-2,2'-disulphonic acid) or inhibition of the lactate transporter with cinnamate. 6. Fibres fatigued in cinnamate displayed a markedly larger acidification (approximately 0.4 pH units) and tension fell more rapidly than under control conditions; inhibition of Na(+)-H+ and HCO3(-)-Cl- exchange did not have any significant effect on fatigue. 7. The intracellular buffer power, assessed by exposing fibres to the weak base trimethylamine, was about 15 mM (pH unit)-1 in a HEPES-buffered solution (non-CO2 or intrinsic buffer power) and about 33 mM (pH unit)-1 in a bicarbonate-buffered solution. Somewhat higher values of the intrinsic buffer power was obtained from changes of the partial pressure of CO2 (PCO2) of the bath solution. Application of lactate or butyrate frequently gave an infinite buffer power, which indicates that powerful pH-regulating mechanisms operate in these cases.(ABSTRACT TRUNCATED AT 400 WORDS)

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Year:  1992        PMID: 1522520      PMCID: PMC1176067          DOI: 10.1113/jphysiol.1992.sp019074

Source DB:  PubMed          Journal:  J Physiol        ISSN: 0022-3751            Impact factor:   5.182


  33 in total

Review 1.  Assessment of Fura-2 for measurements of cytosolic free calcium.

Authors:  M W Roe; J J Lemasters; B Herman
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2.  Movement of acid equivalents across the mammalian smooth muscle cell membrane.

Authors:  C C Aickin
Journal:  Ciba Found Symp       Date:  1988

3.  Intracellular pH measurements in Ehrlich ascites tumor cells utilizing spectroscopic probes generated in situ.

Authors:  J A Thomas; R N Buchsbaum; A Zimniak; E Racker
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4.  Ryanodine receptor of skeletal muscle is a gap junction-type channel.

Authors:  J Ma; M Fill; C M Knudson; K P Campbell; R Coronado
Journal:  Science       Date:  1988-10-07       Impact factor: 47.728

5.  An investigation of the ionic mechanism of intracellular pH regulation in mouse soleus muscle fibres.

Authors:  C C Aickin; R C Thomas
Journal:  J Physiol       Date:  1977-12       Impact factor: 5.182

6.  Lactate and potassium fluxes from human skeletal muscle during and after intense, dynamic, knee extensor exercise.

Authors:  C Juel; J Bangsbo; T Graham; B Saltin
Journal:  Acta Physiol Scand       Date:  1990-10

7.  Intracellular pH and buffer power of type 1 and 2 fibres from skeletal muscle of Xenopus laevis.

Authors:  N A Curtin
Journal:  Pflugers Arch       Date:  1987-04       Impact factor: 3.657

8.  Lactate transport in isolated mouse muscles studied with a tracer technique--kinetics, stereospecificity, pH dependency and maximal capacity.

Authors:  C Juel; F Wibrand
Journal:  Acta Physiol Scand       Date:  1989-09

9.  Changes in tetanic and resting [Ca2+]i during fatigue and recovery of single muscle fibres from Xenopus laevis.

Authors:  J A Lee; H Westerblad; D G Allen
Journal:  J Physiol       Date:  1991-02       Impact factor: 5.182

10.  Slowing of relaxation during fatigue in single mouse muscle fibres.

Authors:  H Westerblad; J Lännergren
Journal:  J Physiol       Date:  1991-03       Impact factor: 5.182

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  41 in total

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Authors:  P D Clarke; D L Clift; M Dooldeniya; C A Burnett; N A Curtin
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6.  Elevated resting H+ current in the R1239H type 1 hypokalaemic periodic paralysis mutated Ca2+ channel.

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7.  Mechanisms underlying reduced maximum shortening velocity during fatigue of intact, single fibres of mouse muscle.

Authors:  H Westerblad; A J Dahlstedt; J Lännergren
Journal:  J Physiol       Date:  1998-07-01       Impact factor: 5.182

8.  Incubation with sodium nitrite attenuates fatigue development in intact single mouse fibres at physiological P O 2 .

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9.  Changes of tension and [Ca2+]i during beta-adrenoceptor activation of single, intact fibres from mouse skeletal muscle.

Authors:  S P Cairns; H Westerblad; D G Allen
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10.  Ca²⁺-pumping impairment during repetitive fatiguing contractions in single myofibers: role of cross-bridge cycling.

Authors:  Leonardo Nogueira; Amy A Shiah; Paulo G Gandra; Michael C Hogan
Journal:  Am J Physiol Regul Integr Comp Physiol       Date:  2013-05-15       Impact factor: 3.619

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