I grepped the adapter sequence to the fastq file with coloring option, and found out that there are a lot of reads that contain adapters. But most of them are on the beginning of the reads(5' end) rather than at the end (3' end).

How is it possible for adapter sequence to be present in the beginning of the reads? I thought the mechanisms of the adapters is that when the sheared mRNA pieces ligated with adapters are shorter than the sequencing length. When the sequence of interest is shorter than the sequencing cycle, machine sequences into the adapter ligated to the 3' end of the each molecule. If this true, we should only expect to see the adapter in the 3'end, correct?

Where do my mental model falls short?

I think it could be due to adapter dimers. Both ends of the fragments (5' and 3') have adapters, but the one at the 5' end is usually not visible in the read sequence because that's where the sequencing process starts. If you have an adapter dimer, however, the polymerase can attach to the first adapter, reading through the second one, if you understand what I mean.