After using tophat I want to count genes with HTSeq and analyse in R with DEseq. But I have a question. I must input all pair-end fastq files of a experimental group once, or run a tophat for each pair-end fastq file?

If you have biological replicates, then you should run tophat for each replicate separately. This is because DEseq uses counts from each biological replicate to estimate the dispersion. I don't think HTseq is smart enough to handle library tags in the BAM file and produce counts for each library separately. Hope it makes sense to you.