Can you give us more information on what sequencing platform? How many reads? What the coverage is? What assembler you used?

Hmmm I'll definetly do that but in a 86Mbp plant genome there can't be many repeats.

Why do you say that?

To follow up on peri4n's response, plant genome size correlates strongly with transposon (LTR retrotransposon, to be specific) copy number. There are also differences in rates of DNA removal between species, but you can bet a small plant genome will have fewer LTR elements than a closely related species with a large genome. There will certainly be some repeats, but 86 Mb is extremely small for a plant genome. Given a size in plants of ca. 5-10 kb, there can't be many LTR elements. http://www.hindawi.com/journals/jb/2010/382732/ http://www.ncbi.nlm.nih.gov/pubmed/20064738

@peri4n: If I were you, I would definitely try another assembler such as SGA and SOAPdenovo. Even the best assembler may behave unexpectedly given data of special features. CLC's assembler, from what I heard, is fast but not the best in terms of accuracy and contiguity. BTW, 60% GC is very high. Illumina will suffer.

@lh3: You are right about ALLPATHS-LG. It sounds like the OP has a range of insert sizes of PEs and mate pairs, but it is not clear if he has the "overlapping paired-end library" required by ALLPATHS.

Sorry I forgot to mention, that I used SSpace for scaffolding. If I remember correctly it is 60% GC.

+1. 60% GC is very high. Illumina will suffer.

@Haibao: I think ALLPATHS-LG always requires libraries with at least 2 distinct insert sizes?