You are correct, despite your confusion! You can have fragments of many sizes. Say there is a 500 bp fragment, and the run is paired-end 100 bp reads. You'll get 100 bp of the left end of the fragment, and 100 bp of the right end of the fragment, and 300 bp of unknown sequence between. If the fragment is 100 bp, you read the same DNA twice, in different directions.

The sequencing starts with a primer hybridizing to the adapter of your template. One nucleotide is added at a time, visualized for incorporation, and the process is repeated for the number of cycles desired (100 bp, 150 bp, etc.).

Thanks a lot!

Another small point is that the piece in between your two 100bp reads is unknown, but we know the two 100bp pieces should align 'somewhere' together. So finding that 'somewhere' is more accurate based on this, resulting in less wasted sequence following alignment.