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Dephosphorylation of MnDPDP and related compounds by acid and alkaline phosphatase.

机译:MnDPDP和相关化合物被酸和碱性磷酸酶脱磷酸。

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摘要

The enzymatic dephosphorylation of the magnetic resonance imaging contrast agent Teslascan was studied in in vitro experiments with acid phosphatase (prostatic, from human semen) and alkaline phosphatase (from human placenta). The active component, MnDPDP (manganese (II)-N,N'-dipyridoxylethylenediamine-N,N'-diacetate-5,5'-bis(phosphate), was dephosphorylated by both enzymes to the monophosphate MnDPMP and the totally dephosphorylated compound MnPLED. The corresponding zinc compound, ZnDPDP (which is a result of in vivo metabolism), was also dephosphorylated by both enzymes to ZnDPMP and ZnPLED. In separate experiments, both enzymes dephosphorylated MnDPMP and ZnDPMP. With the same amount of enzyme units, alkaline phosphatase was almost four times more active than acid phosphatase in dephosphorylating MnDPDP and ZnDPDP with only minor differences whether the substrate contained Mn or Zn. A similar difference in enzymatic activity was seen with the monophosphates, MnDPMP and ZnDPMP. This, taken together with the approximately 50 times higher activity of alkaline phosphatase than acid phosphatase in serum shows that alkaline phosphatase is responsible for most of the dephosphorylation of MnDPDP and its metabolites in vivo.
机译:磁共振成像造影剂Teslascan的酶促去磷酸化已在体外实验中用酸性磷酸酶(来自人精液的前列腺)和碱性磷酸酶(来自人胎盘)进行了研究。两种酶均将活性成分MnDPDP(锰(II)-N,N'-二吡啶氧基乙二胺-N,N'-二乙酸5,5'-双(磷酸))磷酸化为单磷酸MnDPMP和完全脱磷酸的化合物MnPLED相应的锌化合物ZnDPDP(是体内代谢的结果)也被两种酶都去磷酸化为ZnDPMP和ZnPLED;在单独的实验中,这两种酶都对MnDPMP和ZnDPMP进行了磷酸化,而酶单元的量相同,碱性磷酸酶在使MnDPDP和ZnDPDP脱磷酸中,其活性几乎是酸性磷酸酶的四倍,无论底物是Mn还是Zn都只有很小的差异;单磷酸盐MnDPMP和ZnDPMP的酶促活性也有相似的差异,这与大约50血清中碱性磷酸酶的活性是酸性磷酸酶的3倍,表明碱性磷酸酶负责MnDPDP及其代谢物的大部分去磷酸化在体内测试。

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