研究目的
Determine the impact of rod photoreceptor-specific expression of Cre recombinase on the kinetics of phototransduction in the mouse eye and identify changes in gene expression that underlie any observed phenotypic differences.
研究成果
The iCre75 mouse line exhibits accelerated phototransduction inactivation due to overexpression of R9AP, resulting from an aberrant R9AP-expressing transcript. This finding underscores the importance of considering the presence of additional transgenes when designing experiments with this mouse line.
研究不足
The study highlights the presence of an additional R9AP-expressing transgene in the iCre75 mouse line, which must be considered in experimental design. The findings suggest a need for caution when using this mouse line for rod-specific gene loss of function studies.
1:Experimental Design and Method Selection:
Transretinal ERG and single-cell suction electrode recordings were used to measure the kinetics of phototransduction in a mouse line exhibiting rod photoreceptor–specific Cre recombinase expression. Gene expression changes were evaluated using RNA sequencing transcriptome analysis.
2:Sample Selection and Data Sources:
Mice were euthanized after dark adaptation, and retinas were dissected for analysis.
3:List of Experimental Equipment and Materials:
Equipment included a differential amplifier, digitizer, data acquisition software, and a cyan 505-nm LED light. Materials included Ringer’s solution, Leibovitz culture medium L-15, and antibodies for immunoblotting.
4:Experimental Procedures and Operational Workflow:
Retinas were perfused with Ringer’s solution, and light-dependent changes in voltage were measured. RNA was extracted for sequencing, and immunoblotting was performed to evaluate protein levels.
5:Data Analysis Methods:
Data were analyzed using ClampFit and Origin software, with statistical significance determined using a two-tailed Student’s t-test.
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