β-Galactosidases in Ripening Tomatoes

Pressey, Russell

doi:10.1104/pp.71.1.132

Cited by 221 publications

(114 citation statements)

References 14 publications

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“…These data indicate that the partially purified cotyledonary β-gal I, β-gal II and β-gal III extracted from Pitiúba cowpea were heat stable up to 50°C, and that their thermostability is similar to the β-galactosidases isolated from cotyledons of Vigna sinensis (Biswas 1987) and Vigna radiata (Kundu et al 1990), as well as from β-galactosidases isolated from other plants sources (Konno & Katoh 1986, Simos & Georgatsos 1988. However, they differ from the ones obtained with β-galactosidases isolated from radish (Sekimata et al 1989) and tomato seeds (Pressey 1983), which were inactive at 55°C or had only 50% of their initial activities at temperature ranging from 48 to 52°C, respectively.…”

Section: Resultsmentioning

confidence: 75%

“…These results are similar to those found for cotyledonary β-galactosidases from Vigna sinensis (Biswas 1987) and Vigna radiata (Kundu et al 1990), as well as for seeds (Agrawal & Bahl 1968, Li et al 1975, Matheson & Saini 1977 al. 1988, Sekimata et al 1989, Giannakouros et al 1991, Buckeridge & Reid 1994, shoots (Konno & Tsumuki 1993), leaves (Sawicka & Kacperska 1995) and fruits (Pressey 1983, Ogawa et al 1990, Ranwala et al 1992) of different species.…”

Section: Resultsmentioning

confidence: 99%

“…2000Sekimata et al 1989, Simos et al 1989, Kundu et al 1990, Giannakouros et al 1991, Enéas-Filho et al 1995. It has been suggested that these enzymes are associated to the depletion of oligo-and polysaccharides during the initial phases of seed germination (Matheson & Saini 1977, Corchete & Guerra 1986, Biswas 1987, Enéas-Filho et al 1995, involved in the metabolism of cell wall constituints (Corchete & Guerra 1987a, Edwards et al 1988, Dopico et al 1989, Konno & Katoh 1992, Konno & Tsumuki 1993, Gómez et al 1995, Kitagawa et al 1995, and in the process of fruit ripening (Pressey 1983, Ogawa et al 1990, Veau et al 1993, Ali et al 1995. β-galactosidase activity has been detected in quiescent seeds (Dey 1984) as well as during germination and seedling establishment (Agrawal & Bahl 1968, Corchete & Guerra 1987b, Kundu et al 1990, Buckeridge & Reid 1994, Enéas-Filho et al 1995.…”

Section: Resumo -(Múltiplas Formas De β-Galactosidases Cotiledonares mentioning

confidence: 99%

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Multiple forms of cotyledonary b-galactosidases from Vigna unguiculata quiescent seeds

Enéas-Filho¹,

Sudério²,

Gomes-Filho³

et al. 2000

Rev. bras. Bot.

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-(Multiple forms of cotyledonary β-galactosidases from Vigna unguiculata quiescent seeds). Cotyledonary β-galactosidases were isolated and partially purified from Pitiúba cowpea (Vigna unguiculata (L.) Walp.) quiescent seeds. The purification steps consisted of precipitation of the crude extract with ammonium sulphate in the range of 20-60% saturation, acid precipitation, DEAE-Sephadex ion-exchange chromatography and Lactosyl-Sepharose affinity chromatography. This purification process gave rise to three β-galactosidases-rich fractions: β-gal I, β-gal II and β-gal III, which were purified about 5, 509, and 62 fold, respectively. They reached maximal enzyme activity at different pH ranges: 3.5-4.5 for β-gal I, 3.0-3.5 for β-gal II, and 3.0-4.0 for β-gal III. Their maximal activities were reached when the temperature of the assay medium was 60°C, and preincubation of the enzymes at different temperatures has shown that they were heat-stable up to 50°C. There were no significant differences among the partially purified enzymes as to their response to the different effectors tested, except for Mn 2+ and EDTA, which affected β-gal I, β-gal II, and β-gal III differ- other plant β-galactosidases. Although three isoforms of this enzyme were obtained through this purification process, isoelectric focusing in polyacrylamide slab gel of these enzyme-proteins suggests that cotyledons of Pitiúba cowpea quiescent seeds possess four isoforms of β-galactosidases. RESUMO -(Múltiplas formas de β-galactosidases cotiledonares de sementes quiescentes de Vigna unguiculata).β-galactosidases cotiledonárias foram isoladas e purificadas, parcialmente, de sementes quiescentes de feijão-de-corda (Vigna unguiculata (L.) Walp.) Pitiúba. As etapas de purificação consistiram de precipitação do extrato bruto com sulfato de amônio na faixa de 20-60% de saturação, precipitação ácida, cromatografia de troca-iônica em DEAE-Sephadex e cromatografia de afinidade em Lactosil-Sepharose. Esse processo de purificação deu origem a três frações ricas em β-galactosidases: β-gal I, β-gal II e β-gal III, as quais foram purificadas cerca de 5, 509 e 62 vezes, respectivamente. Elas atingiram máxima atividade enzimática em diferentes faixas de pH: 3,5-4,5 para β-gal I, 3,0-3,5 para β-gal II e 3,0-4,0 para β-gal III. Suas atividades máximas foram alcançadas quando a temperatura do meio de ensaio era 60°C, e a preincubação das enzimas em diferentes temperaturas mostrou que elas eram termoestáveis até 50°C. Não houve diferenças significativas entre as enzimas parcialmente purificadas no que respeita à resposta dos diferentes efetores testados, exceto para Mn 2+ e EDTA, que afetaram, diferentemente, β-gal I, β-gal II e β-gal III. . Essas propriedades químicas e físicas são semelhantes às encontradas para outras β-galactosidases de plantas. Embora três isoformas dessa enzima tenham sido obtidas através desse processo de purificação, a focalização isoelétrica em placa de gel de poliacrilamida dessas proteinas enzimáticas sugere que cotilédones de sementes qu...

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Section: Resultsmentioning

confidence: 75%

Section: Resultsmentioning

confidence: 99%

Section: Resumo -(Múltiplas Formas De β-Galactosidases Cotiledonares mentioning

confidence: 99%

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Multiple forms of cotyledonary b-galactosidases from Vigna unguiculata quiescent seeds

Enéas-Filho¹,

Sudério²,

Gomes-Filho³

et al. 2000

Rev. bras. Bot.

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“…The loss of Gal can occur independently of PG activity (Carrington et al, 1993), suggesting the involvement of other classes of enzymes such as ␤-galactosidases/␤-galactanases, which have been associated with many ripening fruits (Ross et al, 1993(Ross et al, , 1994Carey et al, 1995;Lashbrook et al, 1997), and which may act on several classes of polysaccharides, including the galactan side chains of rhamnoglacturonans (Pressey, 1983). Loss of galactans has been demonstrated to accompany or even precede increased solublization of polyuronides (Gross and Wallner, 1979;Kim et al, 1991), and purified or partially purified ␤-galactosidase has been shown to catalyze an apparent decrease in the molecular size of pectins in vitro in tomato (De Veau, 1993) and melon fruits (Ranwala et al, 1992).…”

Section: Na 2 Co 3 -Soluble Fractionmentioning

confidence: 99%

Temporal Sequence of Cell Wall Disassembly in Rapidly Ripening Melon Fruit1

Rose¹,

Hadfield²,

et al. 1998

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The Charentais variety of melon (Cucumis melo cv Reticulatus F1 Alpha) was observed to undergo very rapid ripening, with the transition from the preripe to overripe stage occurring within 24 to 48 h. During this time, the flesh first softened and then exhibited substantial disintegration, suggesting that Charentais may represent a useful model system to examine the temporal sequence of changes in cell wall composition that typically take place in softening fruit. The total amount of pectin in the cell wall showed little reduction during ripening but its solubility changed substantially. Initial changes in pectin solubility coincided with a loss of galactose from tightly bound pectins, but preceded the expression of polygalacturonase (PG) mRNAs, suggesting early, PG-independent modification of pectin structure. Depolymerization of polyuronides occurred predominantly in the later ripening stages, and after the appearance of PG mRNAs, suggesting the existence of PG-dependent pectin degradation in later stages. Depolymerization of hemicelluloses was observed throughout ripening, and degradation of a tightly bound xyloglucan fraction was detected at the early onset of softening. Thus, metabolism of xyloglucan that may be closely associated with cellulose microfibrils may contribute to the initial stages of fruit softening. A model is presented of the temporal sequence of cell wall changes during cell wall disassembly in ripening Charentais melon.Ripening in many fruits is associated with textural changes that are believed to result from disassembly of the primary cell wall. This includes modifications of the structure and composition of the constituent polysaccharides that have been correlated with the expression of a range of hydrolases and transglycosylases (Fischer and Bennett, 1991; Lashbrook et al., 1997) and the potential alteration of covalent and noncovalent interactions between polysaccharide classes. A recent model of the plant primary cell wall described a network of cellulose microfibrils that surrounds the cell and is enmeshed in coextensive matrices of pectic and hemicellulosic polymers, with additional minor components such as structural proteins (Carpita and Gibeaut, 1993). During fruit softening, pectins (Brady, 1987; Fischer and Bennett, 1991) and hemicelluloses (Lashbrook et al., 1997) typically undergo solubilization and depolymerization that are thought to contribute to wall loosening and disintegration, although the relative extent and timing vary between species.

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“…In the combined pectic fraction (Table 111), linkages identified as typical for tomato pectic polysaccharides (based on the report of Pressey [1983] and the thorough analysis of Seymour et al 119901) comprised more than 90% of the total identified linkages. The most abundant linkages were 1,5-arabinosyl (furanosyl) residues (23% of the total), 1,4-galactosyl residues (18% of the total), and terminal galactosyl, and 1,2-and/or 1,4-xylosyl residues (not separable under the chromatographic conditions employed [15% of the total]).…”

Section: Glycosyl Linkage Composition and Labelingmentioning

confidence: 99%

Cell Wall Metabolism in Ripening Fruit (IX. Synthesis of Pectic and Hemicellulosic Cell Wall Polymers in the Outer Pericarp of Mature Green Tomatoes (cv XMT-22)

1997

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Discs of outer pericarp were excised from mature green tomato (Lycopersicon esculentum Mill.) fruit and kept in sterile tissue culture plates for 4 d, including 2 d of incubation with D-[U-'3C]glucose. Cell walls were prepared and the water-soluble, pectic, and hemicellulosic polymers were extracted. Cell wall synthetic capacity was determined by gas chromatography-mass spectrometry analysis of incorporation of the heavy isotope label. l h e "outer" 2-mm pericarp region, which included the cuticle, had a lower cell wall synthetic capacity than the "inner" 2-mm region immediately below it (closer to the locules), based on the percentage of labeling of the neutral sugars. lhere were no significant differences in relative abundance of glycosidic linkages in the two tissue regions. Label was incorporated into neutral sugars and linkages typical for each polysaccharide class were identified in the cell wall preparations. Calacturonic acid and glucuronic acid were labeled to an extent similar to that of the neutral sugars in each tissue region.

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β-Galactosidases in Ripening Tomatoes

Cited by 221 publications

References 14 publications

Multiple forms of cotyledonary b-galactosidases from Vigna unguiculata quiescent seeds

Multiple forms of cotyledonary b-galactosidases from Vigna unguiculata quiescent seeds

Temporal Sequence of Cell Wall Disassembly in Rapidly Ripening Melon Fruit1

Cell Wall Metabolism in Ripening Fruit (IX. Synthesis of Pectic and Hemicellulosic Cell Wall Polymers in the Outer Pericarp of Mature Green Tomatoes (cv XMT-22)

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