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Assessment of decalcifying protocols for detection of specific RNA by non-radioactive in situ hybridization in calcified tissues
Authors:Y. Shibata  S. Fujita  H. Takahashi  A. Yamaguchi  T. Koji
Affiliation:(1) Department of Oral Pathology, Nagasaki University School of Dentistry, 1–7-1 Sakamoto, Nagasaki 852–8588, Japan e-mail: siva@net.nagasaki-u.ac.jp Tel.: +81-95-8497646, Fax: +81-95-8497647, JP;(2) Department of Histology and Cell Biology, Nagasaki University School of Medicine, 1–12-4 Sakamoto, Nagasaki 852–8523, Japan, JP
Abstract:For the best performance of in situ analysis of specific RNA expression in calcified tissues, it is necessary to choose an appropriate protocol to decalcify the tissues. We evaluated the usefulness of various acid-based decalcifying reagents with reference to 28 S rRNA staining by in situ hybridization using a thymine-thymine dimerized oligonucleotide probe. The reagents evaluated were 10% nitric acid, 10% HCl, 5% formic acid, 5% trichloroacetic acid, Morse’s solution, Plank-Rychlo’s solution, and K-CX solution, all of which are commonly used to decalcify tissues, and their effects on retention of morphology and RNA were compared with EDTA-based solutions. When normal mouse mandible was used as a model tissue, well-preserved morphology of ameloblasts was obtained from sections decalcified with Morse’s solution, 10% HCl, Plank-Rychlo’s solution, and K-CX solution, and best retention of 28 S rRNA was obtained with 5% formic acid and Morse’s solution. We recommend Morse’s solution to decalcify tissues to be processed for the rapid analysis of specific RNA expression. Indeed, we detected specific mRNAs strongly in sections treated with Morse’s solution, and quantitative analysis showed that the ratio of signal intensities of 28 S rRNA and the specific mRNAs correlated with each other depending on decalcifying solutions. Accepted: 3 January 2000
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