Velvet + meta-velvet:which fastq format for paired-end infos?

I have been using velvet with the new formats of MiSeq and HiSeq PE data, and it works fine.

By the way, in the read that you have used to illustrate the new format, the Y (1:Y:18:ATCACG) indicates a read that has not passed Illumina's QC filter step.

Usually the sequence providers remove those reads.

Velvet ignores fastq headers and replaces them with its own (fasta) headers anyway. You just have to make sure that input read pairs are either shuffled in one file, or synced if separate files are used.

@mastal
Thanks, but the example reads I've posted are not mine. they are from the wikipedia page illustrating the differences between the fastq-formats.
@mastal+@muol:
But then how can I check the assemblies with regard to paired-end Infomation? With Mira, for example, I know that you still get assemblies (without error-messages) if you use the wrong format. The assemblies will just in reality be based on single-read assemblies. So how can one really make sure if everything is ok, if the paired-end info is left out from the AMOS-file, the sequence-list and everything? (This just intrigues me. For some contigs i would simply like to check how well supported they are by paired reads. Also a lot of reads are not assembled or dropped from the assembly. I would like to see what has happened to their corresponding partners)