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The ACC oxidase (ACO) activity was measured as the ability of plant tissue to convert exogenous ACC to ethylene. The homogenate was prepared in an extraction buffer as described byMoya-Leon and John (1994), with modifications. One g tomato pericarp tissue was homogenized using a cold pestle and mortar with 3mL extraction buffer which contained 0.1MTris¨CHCl (pH7.5), 5%PVP, 10%glycerol, 5.0 mM dithiothreitol, 0.1 mM FeSO4 and 30 mM sodium ascorbate. The homogenate was centrifuged at 10,000¡Ág for 20min at 4 ◦C.The determination of ACO activity was carried out in sealed tubes with a reaction mixture containing 1.8mL of 0.1M Tris¨CHCl buffer (pH 7.5, containing 10% glycerol, 30mM sodium ascorbate, 30mM NaHCO3, 0.1mM FeSO4 and 1.0mM ACC) and 0.2mL of enzyme extract. After being incubated at 30 ◦C for 20 min, 1mL of the gaseous portion was removed and assayed for ethylene as described above. The ACO activity was expressed as nmol g−1 FWh−1.
Extracts for lipoxygenase (LOX) activity assays were prepared according to the method of Surrey (1964), with slight modifications. Two g tomato pericarp tissue was homogenized using a cold pestle and mortar in 10mL of 50mM phosphate buffer (pH 7.0) at 4 ◦C and centrifuged at 10,000¡Ág for 15min. The supernatant liquid was used as the enzyme source. The reaction mixture contained
25 L of 100mM linoleic acid sodium, 2.775mL of 100mM acetic acid buffer (pH 5.5) and 0.2mL of supernatant enzyme extract at 30 ◦C. A unit of LOX was defined as a change of 1 absorbance unit at 234 nm in 1 min using a UVIKON XL Ultraviolet spectrophotometer (Secomam, France).
   These determinations were made from three replicates sampled from 5 fruit.

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ÎôÄê²ÐÃÎ(½ð±Ò+2, ·­ÒëEPI+1): 2011-03-20 13:50:38
The ACC oxidase (ACO) activity was measured as the ability of plant tissue to convert exogenous ACC to ethylene. The homogenate was prepared in an extraction buffer as described by Moya-Leon and John (1994), with modifications.
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2Â¥2011-03-20 13:39:44
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ÎôÄê²ÐÃÎ(½ð±Ò+4): 2011-03-20 13:52:09
One g tomato pericarp tissue was homogenized using a cold pestle and mortar with 3mL extraction buffer which contained 0.1MTris¨CHCl (pH7.5), 5%PVP, 10%glycerol, 5.0 mM dithiothreitol, 0.1 mM FeSO4 and 30 mM sodium ascorbate. The homogenate was centrifuged at 10,000¡Ág for 20min at 4 ◦C.
The determination of ACO activity was carried out in sealed tubes with a reaction mixture containing 1.8mL of 0.1M Tris¨CHCl buffer (pH 7.5, containing 10% glycerol, 30mM sodium ascorbate, 30mM NaHCO3, 0.1mM FeSO4 and 1.0mM ACC) and 0.2mL of enzyme extract.
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ÎôÄê²ÐÃÎ(½ð±Ò+10): 2011-03-20 14:03:54
After being incubated at 30 ◦C for 20 min, 1mL of the gaseous portion was removed and assayed for ethylene as described above. The ACO activity was expressed as nmol g−1 FWh−1.Extracts for lipoxygenase (LOX) activity assays were prepared according to the method of Surrey (1964), with slight modifications. Two g tomato pericarp tissue was homogenized using a cold pestle and mortar in 10mL of 50mM phosphate buffer (pH 7.0) at 4 ◦C and centrifuged at 10,000¡Ág for 15min.
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ÎôÄê²ÐÃÎ(½ð±Ò+14): 2011-03-20 14:11:16
The supernatant liquid was used as the enzyme source. The reaction mixture contained
25 L of 100mM linoleic acid sodium, 2.775mL of 100mM acetic acid buffer (pH 5.5) and 0.2mL of supernatant enzyme extract at 30 ◦C. A unit of LOX was defined as a change of 1 absorbance unit at 234 nm in 1 min using a UVIKON XL Ultraviolet spectrophotometer (Secomam, France).
   These determinations were made from three replicates sampled from 5 fruit.
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