An argyrophil III method for the demonstration of elastic fibres and membranes.

Microscopica acta Pub Date : 1981-03-01
F Gallyas
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Abstract

An esterification with isopropyl alcohol containing 0.2% periodic acid and 2% acetone (at 56 degrees C for 16 hours) followed by a treatment in a special physical developer, similarly, an acetylation with a 3:2 mixture of pyridine and acetic anhydride (at room temperature for 16 hours) followed by the same development, render the elastic fibres and membranes visible. Both pretreatments (esterification and acetylation) serve to make the catalytic points more active in the elastic elements than in the other components of tissue.

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一种展示弹性纤维和膜的argyrophiliii方法。
与含有0.2%周周酸和2%丙酮的异丙醇酯化(在56摄氏度下,16小时),然后在特殊的物理显影剂中处理,类似地,与吡啶和乙酸酐的3:2混合物进行乙酰化(在室温下,16小时),然后进行同样的显影,使弹性纤维和膜可见。两种预处理(酯化和乙酰化)都有助于使弹性元素中的催化点比组织的其他成分更活跃。
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