Properties of alkaline pectate lyase from recombinant strain E.coli JM109(pHsh PL)
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the Chinese National Program for High Technology Research and Development (863-2003AA322050)

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    Abstract:

    Alkaline pectate lyase (PL) from recombinant strain E.coli JM109(pHsh PL)was purified by a three-step process including (NH4)2SO4 precipitation followed by dialysis and chromatography. The purified enzyme appeared homologous on SDS-PAGE. The specific activity of the purified enzyme reached 1079 U/mg. The optimal pH and temperature were in the ranges of pH 9.0 to 10.0 and 50℃ to 66℃. The enzyme was preferable in optimal pH range in enzymatic retting of flax. Enzyme activity slightly increased in the presence of Mg2+ ion, whereas decreased in the presence of other ions, especially Fe2+. The Km of the purified enzyme for polygalacturonic acid was 20.93 mg/L, the Vmax for polygalacturonic acid hydrolysis was 105.3 μmol of unsaturated products per min and Ea was 21.74 kJ/mol. The results of the decay constant (kd ) analysis on condition of PL bonding polygalacturonic acid (kd=0.02 min-1) and PL without polygalacturonic acid ( kd=0.0342 min-1) showed the substrate was helpful to decrease thermal inactivation of PL. The products (unsaturated oligomers) from polygalacturonic acid degraded by PL were analyzed by electrospray ionization mass spectrometry(ESI-MS). The following data were obtained: ESI-MS m/z, 350.82 (unsaturated bigalacturonic acid, uG2), 527.04 (unsaturated trigalacturonic acid, uG3). However, m/z 175 (unsaturated galacturonic acid, uG1) was not found. These results indicate that the final PGA degradation products was a mixture of unsaturated oligo-galacturonides including uG3 and uG2 except for uG1. It suggests that the recombinant PL cannot degrade uG3 and uG2.

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Bin Zhuge, Guocheng Du, Jian Chen. Properties of alkaline pectate lyase from recombinant strain E. coli JM109(pHsh PL). [J]. Acta Microbiologica Sinica, 2008, 48(1): 121-125

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  • Received:May 16,2007
  • Revised:October 16,2007
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