Sarcolemma-specific collagen Ⅵ deficiency can be better demonstrated by double immunofluorescence staining.

Double immunofluorescence staining with monoclonal antibodies(1:100) against phospho-histone H3 and α-sarcomeric actin was performed on the cultured cells.

Methods Cells were harvested at 0 day,the 3rd day and the 7th day after BGSCs differentiation,then the ratio of Hes-1 positive cells were counted by flow cytometry,and the expression intensity and cell types were detected by laser confocal microscopy after immunofluorescence staining with Hes-1 and GFAP,MAP2 or MBP.

The nNOS neurons were detected by immunofluorescence staining.

The aim of this experiment was to study the effective method of fixation and penetration before immunofluorescence staining in oocytes and early embryos to raise the effect of immunofluorescence staining in them.

The purpose of this article is to explore The Organization of cochlear immunofluorescent staining and laser scanning confocal microscope technology applications.

Results Immunofluorescent staining showed predominantly P2X7 and P2X2 receptor expression in OHCs and the distribution of P2X7 receptor overlaped with prestin expression.