You can not convert colorspace to basespace directly. See here why:

An alternative route to using FastQC, which is very nice, is to align first and use the resulting BAM file as input.

Another program I have looked at for duplicate analysis is prinseq, which also offers graphical output.

Did you removed adapter info or trimmed your reads.
what about other fastQC results they are pass or fail.

Some aspects passed and others failed,
I did NO removal of adapters.... Not sure if it was done when i received the csfasta and qual files..
Taking into consideration that this is a direct conversion from color to base space, its understandable that there may be confusing results.... (In all about 45% of reads mapped with color-space-novoAlign to a reference, and only 15% usnig colorspace-tophat/bowtie...)
Any thoughts?
PASS Basic Statistics Corrida_4_FC_1_01_01CVATFR001_F3.fastq
FAIL Per base sequence quality Corrida_4_FC_1_01_01CVATFR001_F3.fastq
WARN Per sequence quality scores Corrida_4_FC_1_01_01CVATFR001_F3.fastq
WARN Per base sequence content Corrida_4_FC_1_01_01CVATFR001_F3.fastq
FAIL Per base GC content Corrida_4_FC_1_01_01CVATFR001_F3.fastq
FAIL Per sequence GC content Corrida_4_FC_1_01_01CVATFR001_F3.fastq
WARN Per base N content Corrida_4_FC_1_01_01CVATFR001_F3.fastq
PASS Sequence Length Distribution Corrida_4_FC_1_01_01CVATFR001_F3.fastq
PASS Sequence Duplication Levels Corrida_4_FC_1_01_01CVATFR001_F3.fastq
PASS Overrepresented sequences Corrida_4_FC_1_01_01CVATFR001_F3.fastq
FAIL Kmer Content Corrida_4_FC_1_01_01CVATFR001_F3.fastq

I would recommend using SAET to clear up any colour errors before alignment. Normally I get 1-5% more aligned reads using this (apparently a lot more with ECC data).

I don't think your fastqc boxplot results are too bad, but I've seen better ones.