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Purification and properties of Manganese Superoxide Dismutase (MnSOD) from Tamarix aphylla L

机译:来自Tamarix aphylla L的锰超氧化物歧化酶(MNSOD)的纯化与性质

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Superoxide dismutase (SOD) of the Tamarix aphylla leaves were detected at optimum conditions that collected in April. May and June. Results indicated the specific activity in the crude extract reaching to 36.76 unit/mg protein. Crude SOD was purified by several techniques, precipitation with ammonium sulfate (50-75)%(,) Ion exchange chromatography using DEAE-cellulose and two steps of size exclusion chromatography on sephacryl S-200 column. The obtained specific activity (310 unit/mg protein) and purification fold 7.91. The purified enzyme revealed one band by SDS-polyacrvlamidc gel electrophoresis with molecular mass 85.703 kDa. while 89.125 kDa by Sephacryl S-200. The optimal pH and temperature for enzyme activity were 7.5. and 50 degrees C respectively. EDTA, SDS and NaN3 reduced activity, contrariwise of H2O2 and KCN, pointed to the studied SOD is MnSOD. Michalis constant K-m and maximum velocity V-max values were 0.016 mM and 55.86 mM/min, respectively by using Pvrogallol as substrate. According to the results, we conclude Tamarix aphylla produce MnSOD which can have purified by serial purification tcchniqucs for better activity and characterized for further studies.
机译:在4月份收集的最佳条件下检测到Tamarix Aphylla叶子的超氧化物歧化酶(SOD)。 5月和6月。结果表明粗提取物中的特定活性达到36.76单位/ mg蛋白。通过几种技术纯化粗糙SOD,使用DEAE-纤维素与硫酸铵(50-75)%(,)离子交换色谱法和Sephacryl S-200柱的大小排阻色谱的两个步骤进行沉淀。获得的特异性活性(310个单元/ Mg蛋白)和纯化折叠7.91。纯化的酶通过SDS-Polyacrvlamidc凝胶电泳显示出一个带,分子量85.703kDa。虽然Sephacryl S-200的89.125 KDA。酶活性的最佳pH和温度为7.5。分别为50℃。 EDTA,SDS和NAN3减少活性,对照的H2O2和KCN依据,指向研究的SOD是MNSOD。 MICHALIS常数K-M和最大速度V-MAX值分别使用PVrogallol作为基材分别为0.016mm和55.86mm / min。根据结果​​,我们得出可通过连续纯化Tcchniqucs纯化的Tamarix Aphylla产生MNSOD,以更好地纯化,并表征进一步研究。

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