Paraffin sections were stained by using standard immunohistochemical procedures described previously. Briefly, mouse tissue samples were fixed with 10% formalin for 24 hrs and paraffin embedded. Four mm thick serial sections were mounted on glass slides and were immunostained with various antibodies described in the previous section following standard procedures39 (link).
Immunostaining for cell signaling proteins
Paraffin sections were stained by using standard immunohistochemical procedures described previously. Briefly, mouse tissue samples were fixed with 10% formalin for 24 hrs and paraffin embedded. Four mm thick serial sections were mounted on glass slides and were immunostained with various antibodies described in the previous section following standard procedures39 (link).
Corresponding Organization :
Other organizations : Fuzhou University
Variable analysis
- Immunocytochemical staining procedures
- Paraffin sections staining
- Detection of target proteins
- Immunostaining of mouse tissue samples
- Seeding of 1 × 10^5 HepG2 cells on a glass slide overnight
- Rinsing with PBS
- Fixation with -20 °C methanol
- Washing with PBS
- Formalin fixation of mouse tissue samples for 24 hrs
- Paraffin embedding of mouse tissue samples
- Mounting of 4 mm thick serial sections on glass slides
- Positive control: Not explicitly mentioned
- Negative control: Not explicitly mentioned
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