In eukaryote cells, messenger RNA (mRNA) processing involves post-transcriptional modification process, 5’-capping, splicing, and 3’ polyadenylation. mRNA binding proteins play important roles in these processes. Previously, we found that a yeast RNA-binding protein, Rbp1p, enhances degradation of mitochondria outer membrane porin mRNA. Under environmental stress conditions, such as glucose deprivation, osmotic stress and heat shock, Rbp1p localizes into cytoplasmic granules, referred to P-bodies. In this thesis, we focus on an interacting protein of Rbp1p, Psp1p. Our current knowledge of Psp1p in Saccharomyces cerevisiae is limit. Structurally, Psp1p comprises three asparagines-rich regions, a glutamine-rich region, and a Psp1-conserved region in its C-terminal. In this work, we found that overexpression of Psp1p not only caused growth inhibition, but also repressed translation. Two-hybrid analysis indicated that Psp1p interacts with a P-body component, the decapping activator Dhh1p. In dhh1△, Psp1p lost its growth inhibition ability, but translation repression property still remained. Moreover, by two-hybrid analysis showed that the C-terminal NMP region of Rbp1p interacted to amino acid 55-216 of Psp1p. Psp1p translocated into cytoplasmic compartments upon glucose deprivation and heat shock, and co-localized with Rbp1p. Psp1p may plays a role in recruitment of Rbp1p recruited to P-bodies under glucose deficient conditions. Finally, Psp1p and Rbp1p may play a role in cell wall maintenance, and Rbp1p probably acted upstream of Psp1p in regulating cell wall integrity.