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猪甲状腺中磷脂酰肌醇的代谢

The metabolism of phosphatidylinositol in the thyroid gland of the pig.

作者信息

Jungalwala F B, Freinkel N, Dawson R M

出版信息

Biochem J. 1971 Jun;123(1):19-33. doi: 10.1042/bj1230019.

Abstract
  1. The metabolism of phosphatidylinositol in pig thyroid has been investigated as a basis for understanding the specific stimulation of the synthesis of this phospholipid in the gland by thyrotropin. 2. The gland contained an active Ca(2+)-dependent phosphatidylinositol-splitting enzyme with an optimum pH of 5.3-5.5. 3. The major water-soluble product (65%) formed by this catabolic enzyme was not phosphorylinositol but a related compound, which may be a cyclic phosphorylinositol. Both this and phosphorylinositol (35%) were released simultaneously from the phosphatidylinositol substrate. 4. The phosphatidylinositol-splitting enzyme was found almost exclusively in the supernatant fraction obtained by homogenization of the gland. It was not present in the acid-phosphatase-containing particulate fraction. 5. The incorporation of [2-(3)H(1)]inositol into phosphatidylinositol in the presence of either CDP-diglyceride or CTP+ATP was most active in the microsomal fraction. 6. When thyroidal microsomes were labelled with [(3)H]inositol and (32)P, and then incubated with unlabelled inositol, there was a dramatic loss of (3)H labelling from the phosphatidylinositol, which was not accompanied by an equivalent loss of (32)P from the phosphate moiety. This turnover of the inositol moiety required nucleotide coenzymes. It is postulated that the phosphatidylinositol is split into inositol and a phosphorus-containing lipid precursor of the phospholipid that remains on the microsomal membrane and is recycled. 7. Isolated thyroidal mitochondria synthesized phosphatidylinositol from [2-(3)H(1)]inositol only because of their contaminating microsomal component. 8. Some evidence has been obtained of a rapid transfer of phosphatidylinositol molecules from thyroidal microsomes to mitochondria when these were incubated together in the presence of a supernatant fraction. 9. Both phosphatidylinositol breakdown by the supernatant fraction of the gland and synthesis by the microsomes were totally inhibited by 1mm-chlorpromazine. This drug is known to suppress thyrotrophin-induced stimulation of activity in thyroid slices.
摘要
  1. 对猪甲状腺中磷脂酰肌醇的代谢进行了研究,以此作为理解促甲状腺激素对该腺体中这种磷脂合成的特异性刺激作用的基础。2. 该腺体含有一种活性钙依赖性磷脂酰肌醇裂解酶,最适pH为5.3 - 5.5。3. 这种分解代谢酶形成的主要水溶性产物(65%)不是磷酸肌醇,而是一种相关化合物,可能是环磷酸肌醇。它和磷酸肌醇(35%)同时从磷脂酰肌醇底物中释放出来。4. 磷脂酰肌醇裂解酶几乎只存在于通过腺体匀浆获得的上清液部分。它不存在于含酸性磷酸酶的颗粒部分。5. 在存在CDP - 甘油二酯或CTP + ATP的情况下,[2 - (3)H(1)]肌醇掺入磷脂酰肌醇的过程在微粒体部分最为活跃。6. 当甲状腺微粒体用[(3)H]肌醇和(32)P标记,然后与未标记的肌醇一起孵育时,磷脂酰肌醇中的(3)H标记显著丢失,而磷酸部分的(32)P没有等量丢失。肌醇部分的这种周转需要核苷酸辅酶。据推测,磷脂酰肌醇被分解为肌醇和一种含磷的磷脂前体,该前体留在微粒体膜上并被循环利用。7. 分离的甲状腺线粒体仅因其污染的微粒体成分而从[2 - (3)H(1)]肌醇合成磷脂酰肌醇。8. 当甲状腺微粒体和线粒体在上清液部分存在的情况下一起孵育时,已获得一些证据表明磷脂酰肌醇分子从甲状腺微粒体快速转移到线粒体。9. 腺体上清液部分对磷脂酰肌醇的分解以及微粒体的合成均被1mmol/L氯丙嗪完全抑制。已知这种药物会抑制促甲状腺激素诱导的甲状腺切片活性刺激。

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A tissue homogenizer.组织匀浆器。
Biochem J. 1960 Nov;77(2):326-7. doi: 10.1042/bj0770326.
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The free myo-inositol of thyroid tissue.甲状腺组织中的游离肌醇。
Proc Soc Exp Biol Med. 1959 Mar;100(3):549-51. doi: 10.3181/00379727-100-24693.

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