I haven’t seen your data and exactly how you did your reads mapping and counting. But please make sure on two things:
First, you use the same version of reference genome at the TopHat step and in your TranscriptDb object.
Second, you specify the right parameters in the reads counting step. They are different for single- vs paired-end data. The workflow example is for paired-end data. Single end data are treated differently:
…
flag <- scanBamFlag(isNotPrimaryRead=FALSE, isProperPair=NA)
param <- ScanBamParam(flag=flag)
gnCnt <- summarizeOverlaps(exByGn, bamfls, mode="Union", ignore.strand=TRUE, single.end=TRUE, param=param)
…

Please check help info for details:
?scanBamFlag
?summarizeOverlaps

Yes I got help in another thread, you are right. Thanks a lot though.
Here is the other thread just if any one wanted to know more.