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Cytochemical localization of malate synthase in amphibian fat body adipocytes: possible glyoxylate cycle in a vertebrate.苹果酸合酶在两栖类脂肪体脂肪细胞中的细胞化学定位:脊椎动物中可能存在的乙醛酸循环
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Localization of enzymes within microbodies.酶在微体中的定位。
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Microperoxisomes in the epithelial cells of the amphibian urinary bladder: an electron microscopic demonstration of catalase and malate synthase.两栖动物膀胱上皮细胞中的微过氧化物酶体:过氧化氢酶和苹果酸合酶的电子显微镜显示
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Glyoxylate cycle in toad urinary bladder: possible stimulation by aldosterone.蟾蜍膀胱中的乙醛酸循环:可能受醛固酮刺激
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9
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10
Subcellular localization of glyoxylate cycle enzymes in Ascaris suum larvae.猪蛔虫幼虫中乙醛酸循环酶的亚细胞定位
J Cell Biol. 1976 Aug;70(2 pt 1):374-83. doi: 10.1083/jcb.70.2.374.

本文引用的文献

1
Development of enzymes in the cotyledons of watermelon seedlings.西瓜幼苗子叶中酶的发育
Plant Physiol. 1973 Jan;51(1):66-71. doi: 10.1104/pp.51.1.66.
2
Isolation of microbodies from plant tissues.从植物组织中分离微体。
Plant Physiol. 1971 Nov;48(5):637-41. doi: 10.1104/pp.48.5.637.
3
Development of Microbodies in Sunflower Cotyledons and Castor Bean Endosperm during Germination.向日葵子叶和蓖麻子胚乳在萌发过程中微体的发育。
Plant Physiol. 1971 Nov;48(5):566-74. doi: 10.1104/pp.48.5.566.
4
Microbodies (Glyoxysomes and Peroxisomes) in Cucumber Cotyledons: Correlative Biochemical and Ultrastructural Study in Light- and Dark-grown Seedlings.黄瓜子叶中的微体(乙醛酸循环体和过氧化物酶体):对光照和黑暗培养幼苗的相关生化及超微结构研究
Plant Physiol. 1971 Oct;48(4):461-75. doi: 10.1104/pp.48.4.461.
5
A "DIRECT-COLORING" THIOCHOLINE METHOD FOR CHOLINESTERASES.一种用于胆碱酯酶的“直接显色”硫代胆碱法。
J Histochem Cytochem. 1964 Mar;12:219-21. doi: 10.1177/12.3.219.
6
[On the catalysis principle of malate synthase].[关于苹果酸合酶的催化原理]
Eur J Biochem. 1967 Jun;1(4):447-75. doi: 10.1111/j.1432-1033.1967.tb00094.x.
7
Association of the glyoxylate cycle enzymes in a novel subcellular particle from castor bean endosperm.蓖麻籽胚乳中一种新型亚细胞颗粒中乙醛酸循环酶的关联
Biochem Biophys Res Commun. 1967 May 25;27(4):462-9. doi: 10.1016/s0006-291x(67)80007-x.
8
Mitochondria and glyoxysomes from castor bean endosperm. Enzyme constitutents and catalytic capacity.蓖麻籽胚乳中的线粒体和乙醛酸循环体。酶成分及催化能力。
J Biol Chem. 1969 Jul 10;244(13):3507-13.
9
Fine structural localization of acyltransferases. The monoglyceride and -glycerophosphate pathways in intestinal absorptive cells.酰基转移酶的精细结构定位。肠道吸收细胞中的甘油单酯和甘油磷酸途径。
J Cell Biol. 1971 Jul;50(1):102-20. doi: 10.1083/jcb.50.1.102.
10
Glyoxysomes of castor bean endosperm and their relation to gluconeogenesis.蓖麻籽胚乳的乙醛酸循环体及其与糖异生的关系。
Ann N Y Acad Sci. 1969 Dec 19;168(2):313-24. doi: 10.1111/j.1749-6632.1969.tb43118.x.

苹果酸合酶在乙醛酸循环体中的细胞化学定位

Cytochemical localization of malate synthase in glyoxysomes.

作者信息

Trelease R N, Becker W M, Burke J J

出版信息

J Cell Biol. 1974 Feb;60(2):483-95. doi: 10.1083/jcb.60.2.483.

DOI:10.1083/jcb.60.2.483
PMID:4130462
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2109154/
Abstract

Cytochemical staining techniques for microbodies (peroxisomes) are limited at present to the enzymes catalase and alpha-hydroxy acid oxidase, and neither technique can distinguish glyoxysomes from other microbodies. Described here is a procedure using ferricyanide for the cytochemical demonstration by light and electron microscopy of malate synthase activity in glyoxysomes of cotyledons from fat-storing cucumber and sunflower seedlings. Malate synthase, a key enzyme of the glyoxylate cycle, catalyzes the condensation of acetyl CoA with glyoxylate to form malate and release free coenzyme A. Localization of the enzyme activity is based on the reduction by free CoA of ferricyanide to ferrocyanide, and the visualization of the latter as an insoluble, electron-opaque deposit of copper ferrocyanide (Hatchett's brown). The conditions and optimal concentrations for the cytochemical reaction mixture were determined in preliminary studies using a colorimetric assay developed to measure disappearance of ferricyanide at 420 nm. Ultrastructural observation of treated tissue reveals electron-opaque material deposited uniformly throughout the matrix portion of the glyoxysomes, with little background deposition elsewhere in the cell. The reaction product is easily visualized in plastic sections by phase microscopy without poststaining. Although the method has been applied thus far only to cotyledons of fat-storing seedlings, it is anticipated that the technique will be useful in localizing and studying glyoxylate cycle activity in a variety of tissues from both plants and animals.

摘要

目前,针对微体(过氧化物酶体)的细胞化学染色技术仅限于过氧化氢酶和α - 羟基酸氧化酶,而且这两种技术都无法将乙醛酸循环体与其他微体区分开来。本文描述了一种使用铁氰化物的方法,通过光镜和电镜对储存脂肪的黄瓜和向日葵幼苗子叶乙醛酸循环体中的苹果酸合酶活性进行细胞化学显示。苹果酸合酶是乙醛酸循环的关键酶,催化乙酰辅酶A与乙醛酸缩合形成苹果酸并释放游离辅酶A。酶活性的定位基于游离辅酶A将铁氰化物还原为亚铁氰化物,以及将后者可视化为不溶性、电子不透明的亚铁氰化铜沉积物(哈奇特棕)。细胞化学反应混合物的条件和最佳浓度是在初步研究中确定的,该研究使用了一种比色测定法来测量420nm处铁氰化物的消失情况。对处理过的组织进行超微结构观察发现,电子不透明物质均匀地沉积在乙醛酸循环体的整个基质部分,而细胞其他部位的背景沉积很少。通过相差显微镜在塑料切片中很容易观察到反应产物,无需进行复染。尽管该方法目前仅应用于储存脂肪的幼苗子叶,但预计该技术将有助于在植物和动物的各种组织中定位和研究乙醛酸循环活性。