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Isoform expression in the multiple soluble malate dehydrogenase of Hoplias malabaricus (Erythrinidae, Characiformes)

A malato desidrogenase solúvel de Hoplias malabaricus (Erythrinidae, Characiformes)

Abstracts

Kinetic properties and thermal stabilities of Hoplias malabaricus liver and skeletal muscle unfractionated malate dehydrogenase (MDH, EC 1.1.1.37) and its isolated isoforms were analyzed to further study the possible sMDH-A* locus duplication evolved from a recent tandem duplication. Both A (A1 and A2) and B isoforms had similar optima pH (7.5-8.0). While Hoplias A isoform could not be characterized as thermostable, B could as thermolabile. A isoforms differed from B isoform in having higher Km values for oxaloacetate. The possibly duplicated A2 isoform showed higher substrate affinity than the A1. Hoplias duplicated A isoforms may influence the direction of carbon flow between glycolisis and gluconeogenesis.

isoforms; sMDH; Hoplias malabaricus; recent locus duplication


A fim de avaliar uma possível duplicação gênica recente no loco sMDH-A* de Hoplias malabaricus, foram analisadas as propriedades eletrocinéticas, cinéticas e de termoestabilidade da malato desidrogenase, estudando-se extratos brutos de fígado e de músculo esquelético, assim como de suas diferentes isoformas isoladas. O efeito do pH sobre a atividade da sMDH mostrou pH ótimo semelhante para as isoformas A (A1 e A2) e B (7.5-8.0). Testes cinéticos de termoestabilidade em H. malabaricus mostram que as isoformas A são mais termoestáveis que as B, mas seus valores de meia-vida não as caracterizam como termoestáveis. Já a isoforma B, pelo valor de meia-vida apresentado, é caracterizada como termolábil. Quanto aos valores de Km para oxalacetato, as isoformas A diferem da isoforma B por apresentarem maiores valores. A presença de duplicação gênica no loco -A*, com a isoforma A2 apresentando maior afinidade com o substrato que a isoforma A1, poderia conferir a essa espécie maior eficiência no processo de redução do oxalacetato a malato, favorecendo o metabolismo no sentido glicolítico.

isoformas; sMDH; Hoplias malabaricus; duplicação lócica recente


Isoform expression in the multiple soluble malate dehydrogenase of Hoplias malabaricus (Erythrinidae, Characiformes)

A malato desidrogenase solúvel de Hoplias malabaricus (Erythrinidae, Characiformes)

Aquino-Silva, M. R.I; Schwantes, M. L. B.II; Schwantes, A. R.II

IUniversidade do Vale do Paraíba, FEAU, Avenida Shishima Hifumi, 2911, CEP 12010-400, São José dos Campos, SP, Brazil

IIUniversidade Federal de São Carlos, Departamento de Genética e Evolução, C.P. 676, CEP 13565-905, São Carlos, SP, Brazil

Correspondence Correspondence to Maria Regina de Aquino-Silva Universidade do Vale do Paraíba, FEAU Avenida Shishima Hifumi, 2911 CEP 12010-400, São José dos Campos, SP, Brazil E-mail: mreginaquino@aol.com

ABSTRACT

Kinetic properties and thermal stabilities of Hoplias malabaricus liver and skeletal muscle unfractionated malate dehydrogenase (MDH, EC 1.1.1.37) and its isolated isoforms were analyzed to further study the possible sMDH-A* locus duplication evolved from a recent tandem duplication. Both A (A1 and A2) and B isoforms had similar optima pH (7.5-8.0). While Hoplias A isoform could not be characterized as thermostable, B could as thermolabile. A isoforms differed from B isoform in having higher Km values for oxaloacetate. The possibly duplicated A2 isoform showed higher substrate affinity than the A1. Hoplias duplicated A isoforms may influence the direction of carbon flow between glycolisis and gluconeogenesis.

Key words: isoforms, sMDH, Hoplias malabaricus, recent locus duplication.

RESUMO

A fim de avaliar uma possível duplicação gênica recente no loco sMDH-A* de Hoplias malabaricus, foram analisadas as propriedades eletrocinéticas, cinéticas e de termoestabilidade da malato desidrogenase, estudando-se extratos brutos de fígado e de músculo esquelético, assim como de suas diferentes isoformas isoladas. O efeito do pH sobre a atividade da sMDH mostrou pH ótimo semelhante para as isoformas A (A1 e A2) e B (7.5-8.0). Testes cinéticos de termoestabilidade em H. malabaricus mostram que as isoformas A são mais termoestáveis que as B, mas seus valores de meia-vida não as caracterizam como termoestáveis. Já a isoforma B, pelo valor de meia-vida apresentado, é caracterizada como termolábil. Quanto aos valores de Km para oxalacetato, as isoformas A diferem da isoforma B por apresentarem maiores valores. A presença de duplicação gênica no loco -A*, com a isoforma A2 apresentando maior afinidade com o substrato que a isoforma A1, poderia conferir a essa espécie maior eficiência no processo de redução do oxalacetato a malato, favorecendo o metabolismo no sentido glicolítico.

Palavras-chave: isoformas, sMDH, Hoplias malabaricus, duplicação lócica recente.

INTRODUCTION

Soluble dimeric malate dehydrogenase (MDH, EC 1.1.1.37) is encoded at two loci – sMDH-A* and sMDH-B*, which results in a three-banded electrophoretic pattern (A2, AB and B2) present in most fish and amphibian species studied (Bailey et al., 1969; Schwantes & Schwantes, 1977, 1982a, b; De Luca et al., 1983; Coppes et al., 1987; Fenerich-Verani et al., 1990; Monteiro et al., 1991, 1998; Farias & Almeida-Val, 1992; Lin & Somero, 1995a, b; Caraciolo et al., 1996; Aquino-Silva et al., 1997).

The subtropical teleost Hoplias malabaricus (Erytrhinidae, Characiformes), studied by Monteiro et al. (1991, 1998), showed a six-banded pattern for sMDH. To explain this pattern these authors suggested a recent locus duplication of sMDH-A* in addition to its sMDH-B*. Since there is no evidence of polyploidy in the Erythrinidae family (Bertollo et al., 1986), and both A-isoforms exhibited a non-divergent pattern of expression and thermostability (Monteiro et al., 1991, 1998; Aquino-Silva et al., 1997) this pattern was explained as the result of regional duplication ("in tandem") occurring at the sMDH-A*. While these sMDH-A* loci encode nondivergent thermostable isoforms, the sMDH-B* encodes a thermolabile one. Adaptation to temperature by the two soluble MDH gene loci of teleost fish, where sMDH-A* encodes a thermostable and sMDH-B* a thermolabile isoform was shown by Schwantes & Schwantes (1982a, b), De Luca et al. (1983), Coppes et al. (1987), Monteiro et al. (1991, 1998), Farias & Almeida-Val (1992), and Lin & Somero (1995a, b).

ln a previous paper (Aquino-Silva et al., 1997) comparing the effect of temperature-pH on liver, muscle and heart unfractionated sMDH of Hoplias, we examined the responses of their apparent Km of oxaloacetate to three temperature assays (10°, 20° and 30°C) and two pH-regimens (temperature-dependent pH and constant-pH imidazole buffer). Liver extracts contributions of duplicate-A thermostable (A1 and A2) and B thermolabile subunits to the isozymes as estimated by Klebe's (1975) method were 16:1, showed the highest Km values, the minimum Km being obtained at 30°C (both pH-regimens). On the other hand, muscle extracts whose A subunit contribution to the isozymes was the smallest among tissues analyzed (2 thermolabile to 1 thermostable), showed the smallest Km values and minimum Km at 10-20°C (temperature-pH dependent and constant-pH imidazole buffer, respectively).

To examine this possible recent gene duplication, the present paper describes optimum pH, thermal stability, and Km (OXA) of total and isolated isoforms of Hoplias sMDH.

MATERIAL AND METHODS

Thirty-one specimens of H. malabaricus were collected by throw net from the Monjolinho Reservoir at the Federal University of São Carlos, State of São Paulo, Brazil. Annual temperature at the H. malabaricus capture site ranges from 12.3°C-23.0°C. Liver and white muscle from each individual were dissected immediately after capture and kept at –20°C. A small piece of each tissue was homogenized (w/v) in a 50 mM phosphate buffer, pH 7.0, using a Potter-Elvejhem tissue homogenizer, and then centrifuged at 19,000 x g for 30 min at 4°C in a Sorvall RC5B centrifuge. Resulting crude extracts were used for electrophoretic and spectrophotometric analyses.

Electrophoreses were carried out in horizontal gels containing 14% (w/v) corn starch prepared according to Val et al. (1981), using the pH 6.9-buffer system described by Whitt (1970). A voltage gradient of 5V/cm was applied for 14-17 h at 4°C. After electrophoresis, the starch gels were sliced lengthwise and the lower halves incubated in an MDH staining solution described by Monteiro et al. (1991). Nomenclature of sMDH gene loci, subunits and iso/allozymes was taken from Shaklee et al. (1989). lsolation of Hoplias MDH isoforms was carried out using an electrophoretic technique according to De Luca et al. (1983).

For studying pH-activity relation, a 50 mM sodium phosphate buffer (pH 5.0-8.5) and a 0.2 mM Tris-HCI buffer (pH 9.0-9.5) were used and assays were carried out in a solution containing 0.33 mM oxaloacetate and 0.20 mM NADH. Crude extracts and isolated isoforms were tested for thermal stability by subjecting each sample to 50°C, for 10-60 min, in absence of substrate or coenzyme. The samples were then cooled on ice and centrifuged at 19.000 x g for 30 min at 4°C. Their residual activities were examined at 25°C in the direction of oxaloacetate reduction through the change in absorbance at 340 nm in a HP-8452A Diode Array Spectrophotometer using a temperature controlled cuvette holder. The assays were carried out in a 50 mM imidazole chloride buffer, containing 0.33 mM oxaloacetate and 0.20 mM NADH. Controls were kept in an ice-water mixture.

The kinetic parameters of sMDH (total and isolated isoforms) were determined at 20°C by measuring the oxidation of NADH spectrophotometrically at 340 nm. The assays were carried out in a 50 mM imidazole chloride buffer containing 0.20 mM NADH and different concentrations of oxaloacetate. Oxamate at 10 mM was added to inhibit lactate dehydrogenase activity resulting from any pyruvate occurring in the assay medium. All assays were performed in triplicate and initiated by adding 10 ml of enzyme (crude extract) or 100 ml (isolated isoform) to 1.0 ml of assay medium. Apparent Michaelis-Menten constants (Km) were calculated by Lineweaver Burk method using double-reciprocal plots of velocity vs substrate concentrations.

Statistical differences among optimum pH, thermal stability, and Km(OXA) values of total and isolated isoforms of Hoplias sMDH were determined by the nonparametric Mann-Whitney test (Zar, 1974) with a probability level of 0.05 chosen as the limit of statistical significance.

RESULTS

Liver and muscle extracts from thirty-one H. malabaricus specimens confirmed the electrophoretic pattern for sMDH, which we previously obtained (Aquino-Silva et al., 1997) in fifty-five other specimens, suggesting the existence of three gene loci: sMDH-B*, sMDH-A1* and sMDH-A2* (Fig. 1A). These latter could be the result of recent locus duplication since both homodimers exhibited a nondivergent pattern of tissue expression. Fig. 1B shows the A1, A2 and B isoforms isolated by electrophoresis.


Comparisons of Hoplias liver and skeletal muscle unfractionated sMDH and its isolated isoforms revealed both similar and diverging kinetic properties between paralogous homologues (encoded by different gene loci in a species) and the nondivergent A-homologues. Both tissues and isolated isoforms showed similar pH optima for oxaloacetate reduction (pH 7.5-8.0) (Fig. 2). Statistical analyses of optimum pH values differed significantly only when liver, and muscle extracts, A1 and A2 versus B isoforms (L x B; M x B; A2 x B; A2 x B, p = 0.0286, respectively), were compared.


Thermal stability of unfractionated sMDH from liver and skeletal muscle extracts is shown in Fig. 3A. When samples were submitted to 50°C for various time periods in the absence of substrate or coenzyme, then assayed at 25°C, the half-life of liver extract, where the thermostable isoform predominates, was about 1 hr while that of skeletal muscle, where the thermolabile isoform predominates, was about 34 min. To determine more precisely the thermal stability of A and B isoforms, partially purified isoforms were also submitted to thermostability tests (Fig. 3B). The half-lives of A1 and A2 isoforms were about 34 min and 16 min, respectively. In this case, isolated A2 isoforms exhibited differences in thermal stability when compared with liver unfractionated crude extracts from which they were isolated. For the B isoform, the half-life was about 4 min. Significant differences were observed among all the half-lives here obtained except when muscle extracts and A1 isoform values (p > 0.9999) were compared.



The responses of both crude extracts and their respective predominant isoforms to various oxaloacetate concentrations are shown in Fig. 4. Optimal substrate concentration differed between isoforms and tissues: A2 isoform has lower optimum concentration for oxaloacetate (0.20 mM L–1) than A1 and B isoforms (0.30 mM L–1 and 0.25 mM L–1); liver extract has higher optimum concentration for oxaloacetate (0.15 mM L–1) than muscle extract (0.04 mM L–1). Statistical analyses of optimal substrate concentration only differ significantly when liver versus A2 isoform (p = 0.1143), and A1 and A2 versus B isoforms (p = 0.1143 and p = 0.200, respectively) were compared. Km of oxaloacetate was higher for liver extracts (0.050 mM L–1) and their A1 and A2 isoforms (0.061 – 0.042 mM L–1) than for muscle extracts (0.014 mM L–1) and their B isoform (0.024 mM L–1).


All the statistical analyses of Km values showed significant differences.

DISCUSSION

New enzymes can be formed since the presence of redundant copies allows one sequence to mutate freely and acquire new catalytic functions. The duplicate genes may have two kinds of homology: orthology and paralogy. Duplicate genes related by speciation are orthologous and genes related by regional events or duplication of a single gene through ploidy changes are paralogous (Ferris, 1984). The homologies of duplicated genes can be inferred from measurements of pH optima, heat stability and other kinetic properties like optimum substrate concentration or Km values.

Two different processes lead to gene duplication. Firstly, a polyploidization where the entire genome is duplicated may occur simultaneously. Secondly, duplication in tandem, involving a single gene locus or several gene loci of a group in linkage, results in gene duplication.

According to Ohno (1970), these two processes complement each other in producing significant gene duplication. According to Bertollo et al. (1986), the Erythrinidae family has shown greatly varying karyotypes, with diploid ranging from 39 to 42 chromosomes and variable chromosomal rearrangements during its evolutionary history. Therefore, in Hoplias, gene duplication could have arisen by tandem duplication (Monteiro et al., 1991, 1998; Aquino-Silva et al., 1997).

Generally, specific activity, thermostability and other kinetic enzyme properties vary with pH fluctuation. De Luca et al. (1983), studying adaptative features of sMDH in the subtropical fish, Astyanax fasciatus, showed that its isoforms had different pH optima for oxaloacetate reduction, being higher for B-thermolabile (7.8 versus 6.5). Otherwise, in comparative studies of sMDH paralogous homologues of four species of Pacific barracudas adapted to different temperatures, Lin & Somero (1995b) obtained, for both isoforms, in the direction of oxaloacetate reduction, similar optima pH (7.6 and 7.7). For Hoplias, optimum pH obtained with muscle and liver extracts, and A1 and A2 isoforms (8.0) was significantly different of the obtained with B isoforms (7.5).

Temperature adaptation by the two paralogous soluble MDH gene loci, where the sMDH-A* encodes a thermostable and the sMDH-B* a thermolabile isoform (Schwantes & Schwantes, 1982a, b; De Luca et al., 1983; Coppes et al., 1987; Farias & Almeida-Val, 1992; Lin & Somero, 1995a, b; Caraciolo et al., 1996) was also detected in H. malabaricus when its unfractionated sMDH was repeatedly incubated at 58°C, electrophoresed and stained for MDH activity (Monteiro et al., 1991, 1998; Aquino-Silva et al., 1997).

However, when isolated A isoforms were incubated to 50°C, for 10-60 min, in the absence of substrate or coenzyme, and assayed for residual activity, they did not exhibit the thermal stability observed through electrophoresis. Comparative studies of thermostable and thermolabile sMDH isoforms of barracuda species from different physiological temperature ranges revealed similar kinetic properties for orthologous and varying for paralogous homologues (Lin & Somero, 1995a, b). According to these authors, the absence of thermolabile isoform in equatorial barracuda (Sphyraena ensis) could occur through two mechanisms: loss of the gene (or functional form of the gene) encoding this isoform, or repression of gene transcription at high temperatures. Thus, if the thermolabile isoform is not required physiologically, the gene encoding this isoform may effectively be lost. However, Farias & Almeida-Val (1992) and Caraciolo et al. (1996) studying the sMDH of Amazon fishes detected the product of the thermolabile locus. Farias & Almeida-Val (1992) also showed a recent duplication of sMDH-B* in Amazon cichlids. Schwantes & Schwantes (1982a), studying the adaptative features of sMDH loci from temperate estuarine fish, Leiostomus xanthurus (habitat temperature range 5-30°C), showed that A and B subunits occur in different tissues at different levels which may be altered by environmental temperature fluctuation. On the other hand, Lin & Somero (1995a, b) studying the eurythermal Gillichthys mirabilis (habitat temperature range 9-38°C), showed that the two isoforms of sMDH vary in ratio seasonally and as a result of acclimation. According to these authors, the findings suggest that temperature can affect one or more of the processes that establish sMDH isozyme ratios, like gene transcription or protein degradation.

Thermostability tests realized with liver extracts, tissue in which Klebe's tests showed the presence of 16 A subunits for 1 of B according to Aquino-Silva et al. (1997), showed the enzyme half-life with 60 minutes of incubation. However, when the isolated A1 and A2 isoforms were incubated, their half-lives were 34 and 16 minutes, respectively. These results showed that the A isoforms could not be seen as the L. xanthurus (Schwantes & Schwantes, 1982a, b) or the Astyanax fasciatus (De Luca et al., 1983) thermostable isoforms (half-lives were well over 1 hr) and showed the first divergence between them: A2 isoform was significantly more thermolabile than A1 isoform. For skeletal muscle extracts, tissue where the sMDH-B* predominates (2 B subunits for 1 A subunit) showed a 34 min and its specific B isoform a 4 min half-lives. According to Lin & Somero (1995b), some characteristics are conserved among orthologous homologues of each sMDH isoform. Comparisons of orthologous homologues with respect to thermostability showed that while A isoforms of H. malabaricus could not be characterized as thermostable isoform, B could be thermolabile.

Studies of orthologous homologues of proteins from species adapted to different temperatures have revealed strong conservation of many kinetic properties (like Km substrate or cofactor) within physiological temperature ranges (Somero, 1978; Hochachka & Somero, 1984; Coppes & Somero, 1990; Lin & Somero, 1995a, b; Aquino-Silva et al., 1997). In eurythermal ectotherms especially species with standing high temperatures, effects of temperature on Km values are generally much smaller than those noted for homologous enzymes of stenothermal species (Baldwin & Aleksiuk, 1973; Coppes & Somero, 1990; Somero, 1981). According to Lin & Somero (1995b), a mechanism by which a eurythermal species might conserve enzymatic function over a wide temperature range is the presence of multiple forms like the sMDH isoforms; not only the two paralogous sMDH differ in thermal stability, but temperature effects on Km values differ among isoforms. Therefore, adaptation to temperature by sMDH in teleosts differs from the pattern obtained for A4-LDH in barracudas (Lin & Somero, 1995b). While in A4-LDH the Km conservation at physiological temperatures came about through evolutionary change in the aminoacid sequence of orthologous homologues, for sMDH conservation may result from altering the ratio of thermostable and thermolabile paralogous isozymes (Lin & Somero, 1995b). ln the present paper, the Km(OXA) values obtained for both A1 and A2 isoform, isolated from liver extract (16A: 1B subunit ratio), were 1.45 higher for A1 isoform (0.061 mM x 0.042 mM), and 2.54 lower than that obtained for B isoform (0.061 mM x 0.024 mM). When we compare the Km isoform values with those obtained for crude extracts in skeletal muscle the Km values are similar to the specific isoform B. Also the Km values for liver extracts are similar to the A1 and A2 isoforms. ln both case, Km values agree with the contributions of gene duplication detected by Aquino-Silva et al. (1997). Also, comparing the Km values shown by H. malabaricus with those obtained from other fishes, we suggest that the A1 isoform of Hoplias could be an orthologous homologues of the A isoform from Geophagus brasiliensis (Aquino-Silva et al., in prep), A. fasciatus (De Luca et al., 1983), L. xanthurus (Schwantes & Schwantes, 1982b), as well as from different species of Pacific barracudas (Lin & Somero, 1995b). The Hoplias B isoform could also be an orthologous homologues of the B1 isoform from G. brasiliensis (Aquino-Silva et al., in prep), and B isoform from A. fasciatus (De Luca et al., 1983), L. xanthurus (Schwantes & Schwantes, 1982b), as well as from the barracudas (Lin & Somero, 1995b).

According to Bailey et al. (1970), the distribution of sMDH isoforms in ectotherms showed certain tissue specificity but its physiological significance has not yet been established. For diverse sMDH isoforms, the less anodic, generally the A isoform is found to some extent in all tissues and B isoform predominates in skeletal muscle (Clayton et al., 1975). Three different biological functions have been proposed for sMDH: gluconeogenesis, lipogenesis and malate-aspartate shuttle during aerobic glycolysis. Since these processes are carried out differently by different tissues, this might be a possible explanation for the different activities of multiple forms of MDH. Their presence or absence would be due to different physiological and metabolic roles. Physiological activities of organisms are influenced by environmental factors such as temperature, dissolved gases, light, pressure, salinity, etc. Thus, development of homeokinetic mechanisms in many organisms could minimize the effects of parametric fluctuation. According to Shaklee et al. (1977), metabolic reorganization during thermal acclimation can be and probably is a tissue-specific process. According to Coppes et al. (1987), the presence of the A isoform in most tissues, more thermostable and more resistant to substrate than the B ones could be correlated with temperature. Both sMDH isoforms may differently affect the carbon flow balance through glycolysis and gluconeogenesis. When temperature increases, metabolic activity increases too, and oxaloacetate would be reduced to malate by A isoform, yielding NAD, which would be used by glyceraldehyde-3-phosphate dehydrogenase, favoring the glycolytic direction. In this case, in the characiform H. malabaricus, the presence of the A2 isoform arisen by gene duplication, would broaden this metabolic pathway, once it showed lower Km value, consequently higher substrate affinity than the A1 isoform.

Acknowledgments — Research supported by Conselho Nacional de Desenvolvimento Científico e Tecnológico (CNPq), and Fundação de Amparo à Pesquisa do Estado de São Paulo (FAPESP). The authors wish to thank Dr. Paula Ann Matvienko-Sikar, who critically reviewed this manuscript. Publication supported by FAPESP.

Received January 23, 2002 – Accepted May 6, 2002 – Distributed February 28, 2003

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  • Correspondence to

    Maria Regina de Aquino-Silva
    Universidade do Vale do Paraíba, FEAU
    Avenida Shishima Hifumi, 2911
    CEP 12010-400, São José dos Campos, SP, Brazil
    E-mail:
  • Publication Dates

    • Publication in this collection
      14 Aug 2003
    • Date of issue
      Feb 2003

    History

    • Accepted
      06 May 2002
    • Received
      23 Feb 2002
    Instituto Internacional de Ecologia R. Bento Carlos, 750, 13560-660 São Carlos SP - Brasil, Tel. e Fax: (55 16) 3362-5400 - São Carlos - SP - Brazil
    E-mail: bjb@bjb.com.br