Preventing arginine-to-proline conversion in a cell-line-independent manner during cell cultivation under stable isotope labeling by amino acids in cell culture (SILAC) conditions |
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| Authors: | Lössner Christopher Warnken Uwe Pscherer Armin Schnölzer Martina |
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| Affiliation: | aGynaeimmunology and Oncology Group, YCR and Liz Dawn Pathology and Translational Sciences Centre, Leeds Institute of Molecular Medicine, St. James’s University Hospital, Leeds LS9 7TF, UK;bDepartment of Histopathology, Institute of Oncology, St. James’s University Hospital, Leeds LS9 7TF, UK |
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| Abstract: | Laser capture microdissection of frozen tissue sections allows homogeneous cell populations to be isolated for expression profiling. However, this requires striking a balance between retaining adequate morphology for accurate microdissection and maintaining RNA integrity. Various staining protocols were applied to frozen endometrial carcinoma tissue sections. Although alcohol-based methods were superior to aqueous stains for maintaining RNA integrity, they suffered from irreproducible staining intensity. We developed a modified alcohol-based, buffered cresyl violet staining protocol that provides reproducible staining with minimal RNA degradation suitable for tissues with moderate to high levels of intrinsic RNase activity. |
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