I am working on an experiment where the Genes of interest were not significantly expressed after the DESeq2 analysis. I applied the filter of 0.05 significance p-value and the genes did not appear. The important genes had a p-value of 1. Is there anything else that could be done as a Bioinformatician to proceed with the analysis?

Edit: My experiment design consists of a control and 2 mutation types. I tried to create DESeq2 conditions MA vs WT and MD vs WT. I am getting upregulated and downregulated genes but it does not consist of the genes that I am interested in. The genes that I am interested in had a log fold change value between 0 and -1 and an adjusted p-value of 1

p-value "hacking" is discouraged and can leave you chasing ghosts when you try to experimentally validate or follow-up on your findings. Without knowing anything about the experimental design, the only real advice I can give is that there is a chance the experiment lacks the power to detect what could be a rather small magnitudinal change in expression between conditions.

I can't say that it is frequent for me to see a p-value of 1 (as well as p-value of 0). It can be that the read counts are too small or p-value is 1 after multiple test correction. Are you sure that you refer to p-value and not to q-value? Are you sure that you used a double-sided test (so you have not mis-specified in which group the expression expected to be elevated)? Could it be that your cases/controls come from different batches and the batch correction was overly aggressive? Can it be that your case/control status somewhat leaked into your design matrix of predictors?

I agree with Jared Andrews - every failed experiment requires a careful autopsy, and without knowing the details it is difficult to perform it.