Comparison of different methods to obtain and store liver biopsies for molecular and histological research.

Gaby Hoffmann, Jooske Ijzer, Bas Brinkhof, Baukje A Schotanus, Ted S G A M van den Ingh, Louis C Penning, Jan Rothuizen
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引用次数: 17

Abstract

Background: To minimize the necessary number of biopsies for molecular and histological research we evaluated different sampling techniques, fixation methods, and storage procedures for canine liver tissue. For addressing the aim, three biopsy techniques (wedge biopsy, Menghini, True-cut), four storage methods for retrieval of RNA (snap freezing, RNAlater, Boonfix, RLT-buffer), two RNA isolation procedures (Trizol and RNAeasy), and three different fixation protocols for histological studies (10% buffered formalin, RNAlater, Boonfix) were compared. Histological evaluation was based on hematoxylin-eosin (HE) and reticulin (fibrogenesis) staining, and rubeanic acid and rhodanine stains for copper. Immunohistochemical evaluation was performed for cytokeratin-7 (K-7), multidrug resistance binding protein-2 (MRP-2) and Hepar-1.

Results: RNA quality was best guaranteed by the combination of a Menghini biopsy with NaCl, followed by RNAlater preservation and RNAeasy mini kit extraction. These results were confirmed by quantitative RT-PCR testing. Reliable histological assessment for copper proved only possible in formalin fixed liver tissue. Short formalin fixation (1-4 hrs) improved immunohistochemical reactivity and preservation of good morphology in small liver biopsies.

Conclusion: At least two biopsies (RNAlater and formalin) are needed. Since human and canine liver diseases are highly comparable, it is conceivable that the protocols described here can be easily translated into the human biomedical field.

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为分子和组织学研究获取和保存肝活组织标本的不同方法的比较。
背景:为了减少分子和组织学研究所需的活检次数,我们评估了犬肝组织的不同采样技术、固定方法和储存程序。为了解决这一问题,我们比较了三种活检技术(楔形活检、Menghini活检、True-cut活检)、四种提取RNA的储存方法(快速冷冻、RNAlater、Boonfix、RLT-buffer)、两种RNA分离方法(Trizol和RNAeasy)以及三种不同的组织学研究固定方案(10%缓冲福尔马林、RNAlater、Boonfix)。组织学评价采用苏木精-伊红(HE)和网状蛋白(纤维生成)染色,铜染色采用红豆酸和罗丹宁染色。免疫组化评价细胞角蛋白-7 (K-7)、多药耐药结合蛋白-2 (MRP-2)和肝素-1。结果:蒙氏活检与NaCl联合使用,rnaalater保存和RNAeasy迷你试剂盒提取是保证RNA质量的最佳方法。这些结果经定量RT-PCR检测证实。对铜的可靠组织学评估证明,只有在福尔马林固定的肝组织中才有可能。短时间的福尔马林固定(1-4小时)改善了免疫组织化学反应性,并在小肝活检中保存了良好的形态学。结论:至少需要两次活检(RNAlater和福尔马林)。由于人类和犬的肝脏疾病具有高度可比性,可以想象,这里描述的方案可以很容易地转化为人类生物医学领域。
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