yes you have made the correct observation, they are basically one in the same except in the latter you walk away a new reference from your consensus

Building your sequence de novo generally requires higher coverage, and you'll end up with lots of contigs that can't be bridged due to repetitive or non-complex sequence. Aligning to a very closely related genome will allow you to easily find discrepancies, even if coverage is not so great. If your coverage is, say, an even 5x, you could call a lot of SNPs. I've found plenty of real, sanger-verified SNPs with 3x coverage. But no de novo assembler will do anything with that.

Also, for a lot of applications, what you really want are the discrepancies between your sample and a reference, so aligning to that reference is a much easier way to find them, rather than building a de novo sample reference, and comparing that to something. Also, de novo won't be totally accurate if your sample is heterozygous, or a mix of samples; at least not Velvet, which is a popular one, and the one I'm most familiar with. Whereas with an aligner, it isn't hard to see that so many reads show one allele at a locus, and so many reads show another.

Very detailed explanation. Thanks for all the responses.

I'm also using Velvet for sequence assembling. How to visualize the Velvet results? There are a lot of result files from Velvet assembling. How to deal with these files?