首页> 外文期刊>Journal of bacteriology >Folic acid and pterin deaminases in Dictyostelium discoideum: kinetic properties and regulation by folic acid, pterin, and adenosine 3',5'-phosphate.
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Folic acid and pterin deaminases in Dictyostelium discoideum: kinetic properties and regulation by folic acid, pterin, and adenosine 3',5'-phosphate.

机译:盘基网柄菌中的叶酸和蝶呤脱氨基酶:动力学特性和叶酸,蝶呤和3',5'-磷酸腺苷的调控。

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Kinetic data obtained for deamination of pterin by the extracellular fraction from Dictyostelium discoideum yielded apparently linear Lineweaver-Burk plots for pterin. The Michaelis constant for pterin was 30 microM. The data for folic acid deamination yielded convex Lineweaver-Burk plots. Convex Lineweaver-Burk plots could result from the presence of two types of enzymes with different affinities. The data for folic acid deamination were analyzed mathematically for two types of enzymes. This analysis produced Michaelis constants for folic acid of 1.8 and 23 microM competition studies suggested that an enzyme with low affinity nonspecifically catalyzed the deamination of folic acid and pterin, whereas an enzyme with high affinity was a specific folic acid deaminase. A specific folic acid deaminase with high affinity appeared to be present on the surface of D. discoideum cells. The Michaelis constant for this enzyme was 2.6 microM. Cells growing in nutrient broth and cells starved in phosphate buffer released folic acid and pterin deaminases. The quantity of deaminase activities released by the cells appeared to be controlled by chemoattractants. Starving cells that were supplied with folic acid, pterin, or adenosine 3',5'-phosphate increased their extracellular folic acid and pterin deaminase activities to a larger extent than did cell suspensions to which no chemoattractants were added. Administration of folic acid or pterin to starving cells caused increases of the activity of extracellular adenosine 3',5'-phosphate phosphodiesterase and repressed increases of the activity of phosphodiesterase inhibitor.
机译:从Disctyostelium Discoideum的细胞外部分脱氨蝶呤获得的动力学数据得出了蝶呤的线性Lineweaver-Burk图。蝶呤的米氏常数为30 microM。叶酸脱氨的数据得出凸的Lineweaver-Burk图。凸Lineweaver-Burk图可能是由于存在两种具有不同亲和力的酶而导致的。对两种类型的酶进行了叶酸脱氨的数据进行了数学分析。该分析得出叶酸的Michaelis常数为1.8和23 microM。竞争研究表明,低亲和力的酶非特异性地催化叶酸和蝶呤的脱氨反应,而高亲和力的酶则是特定的叶酸脱氨酶。具有高亲和力的特定叶酸脱氨酶似乎存在于D. discoideum细胞表面。该酶的米氏常数为2.6 microM。在营养肉汤中生长的细胞和在磷酸盐缓冲液中饥饿的细胞释放叶酸和蝶呤脱氨基酶。细胞释放的脱氨酶活性的数量似乎受趋化因子控制。与未添加化学引诱剂的细胞悬液相比,供应有叶酸,蝶呤或3',5'-磷酸腺苷的饥饿细胞增加了其细胞外叶酸和蝶呤脱氨酶的活性。给饥饿的细胞施用叶酸或蝶呤引起细胞外腺苷3',5'-磷酸磷酸二酯酶活性的增加,并且抑制了磷酸二酯酶抑制剂活性的增加。

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