I would like to know two things

1- why when I look at the ebi.uk for a sample, the fastq files are split in two part for each sample?

2- how to identify if a data is single end or paird reads?for example, I only know Illumina HiSeq 2000 (Homo sapiens). Is there a way to know that?

3- how to know if a the fastq is forward reads or reverse reads and why one should generate that?

thanks

1- why when I look at the ebi.uk for a sample, the fastq files are split in two part for each sample?

A :- These are two pairend reads of one sample that is forward read and reverse reads

2- how to identify if a data is single end or paird reads?

A:- if you have two reads designated for example sample1_1 and sample1_2 or cell1_1 and cell1_2 then its a pairend reads if this is one than its a single end reads

3- how to know if a the fastq is forward reads or reverse reads and why one should generate that?

A:-While downloading fastq file look lines which starts with @ this line has information 1 or 2 in the end of this lines so 1 then its reverse if it 2 then its forward