It all depends on how you are doing the test for differential gene expression. But the basic idea is around statistical power and significance. Generally speaking, you cannot compare one replicate for treatment A with one replicate for treatment B since you have zero statistical power. Even 2 replicates is generally considered not enough since there is a lot of biological and technical variation involved. Most people suggest at least 3 replicates per condition. Then you need to use a principled statistical method to determine differential expression such as the one's incorporated in the packages edgeR or DESeq2. You can't really use simplistic tests like a t-test with RNA-seq data.