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Effect of Immunohistochemistry on Molecular Analysis of Tissue Samples: Implications for Microdissection Technologies
Authors:Michael A. Tangrea   Sumana Mukherjee   Bing Gao   Sanford P. Markey   Qiang Du   Michael Armani   Matthew S. Kreitman   Alex M. Rosenberg   Benjamin S. Wallis   Franziska C. Eberle   Francesca C. Duncan   Jeffrey C. Hanson   Rodrigo F. Chuaqui   Jaime Rodriguez-Canales   Michael R. Emmert-Buck
Abstract:Laser-based tissue microdissection is an important tool for the molecular evaluation of histological sections. The technology has continued to advance since its initial commercialization in the 1990s, with improvements in many aspects of the process. More recent developments are tailored toward an automated, operator-independent mode that relies on antibodies as targeting probes, such as immuno–laser capture microdissection or expression microdissection (xMD). Central to the utility of expression-based dissection techniques is the effect of the staining process on the biomolecules in histological sections. To investigate this issue, the authors analyzed DNA, RNA, and protein in immunostained, microdissected samples. DNA was the most robust molecule, exhibiting no significant change in quality after immunostaining but a variable 50% to 75% decrease in the total yield. In contrast, RNA in frozen and ethanol-fixed, paraffin-embedded samples was susceptible to hydrolysis and digestion by endogenous RNases during the initial steps of staining. Proteins from immunostained tissues were successfully analyzed by one-dimensional electrophoresis and mass spectrometry but were less amenable to solution phase assays. Overall, the results suggest investigators can use immunoguided microdissection methods for important analytic techniques; however, continued improvements in staining protocols and molecular extraction methods are key to further advancing the capability of these methods.
Keywords:immunostaining   immunohistochemistry   proteomics   DNA   RNA   tissue microdissection   expression microdissection   immuno-LCM
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