Abstract
MicroRNAs have subtle and combinatorial effects on the expression levels of their targets. Studying the consequences of a single microRNA knockout often proves difficult as many such knockouts exhibit phenotypes only under stress conditions. This has led to the hypothesis that microRNAs frequently act as buffers of noise in gene expression. Observing and understanding buffering effects requires quantitative analysis of microRNA and target expression in single cells. To this end, we have employed single molecule fluorescence in situ hybridization, immunofluorescence, and high-resolution confocal microscopy to investigate the effects of miR-9a loss on the expression of the serine-protease rhomboid in Drosophila melanogaster early embryos. Our single-cell quantitative approach shows that rhomboid mRNA exhibits the same spatial expression pattern in WT and miR-9a knockout embryos, although the number of mRNA molecules per cell is higher when miR-9a is absent. However, the level of rhomboid protein shows a much more dramatic increase in the miR-9a knockout. Specifically, we see accumulation of rhomboid protein in miR-9a mutants by stage 5, much earlier than in WT. The data therefore show that miR-9a functions in the regulation of rhomboid activity by both inducing mRNA degradation and inhibiting translation in the blastoderm embryo. Temporal regulation of neural proliferation and differentiation in vertebrates by miR-9 is well-established. We suggest that miR-9 family microRNAs are conserved regulators of timing in neurogenic processes. This work shows the power of single-cell quantification as an experimental tool to study phenotypic consequences of microRNA mis-regulation.