I think a more serious issue with your project is demonstrating that the transcripts are not translated. You would need ribosome profiling data to show that there is an absence of translation for those transcripts.

Any experienced scientist cannot advice you to go without experimental validation of some kind. However, I do think you can publish these results without it. Try some of the less rigorous journals like PlosOne (http://www.plosone.org/) and act based on reviewers' comments.

Hi thanks for you feedback,

I may have to explain better, sorry, I already got an experimental collaborator I just used this public data because we got a very close species of the same genera, and since we don't have enough money (yes, we do have money to host a world cup, but the investment on research is being cut, sad..) to do a large scale prediction trough rna-seq and qPCR of or own species, so I thought about using public data to detect ncRNAs in large scale on a close related bacterium and then choose a few ones that are similar on the species we got to validate through qPCR, because qPCR is really expansive I wanted to have more confidence before doing it, to not waste any money. I just didn't wanted to "waste" this result, since a lot of predicted ncRNA where not annotated on this bacterium and the public data is very complete (data on different stages of development with replicates), so I also did differential expression through stages of development. I thought about putting these results together as a methodology in our final paper, but the discussion on two different species would be very confusing to just one paper imo (one with rna-seq differential expression without qpcr, other with just qpcr validation), so I was looking to do two papers. Thank you for your feedback.

Hi Josh, Thank you for your feedback.

I explained it better on Charles Answer, I will just paste it here.

I may have to explain better, sorry, I already got an experimental collaborator I just used this public data because we got a very close species of the same genera, and since we don't have enough money (yes, we do have money to host a world cup, but the investment on research is being cut, sad..) to do a large scale prediction trough rna-seq and qPCR of or own species, so I thought about using public data to detect ncRNAs in large scale on a close related bacterium and then choose a few ones that are similar on the species we got to validate through qPCR, because qPCR is really expansive I wanted to have more confidence before doing it, to not waste any money. I just didn't wanted to "waste" this result, since a lot of predicted ncRNA where not annotated on this bacterium and the public data is very complete (data on different stages of development with replicates), so I also did differential expression through stages of development. I thought about putting these results together as a methodology in our final paper, but the discussion on two different species would be very confusing to just one paper imo (one with rna-seq differential expression without qpcr, other with just qpcr validation), so I was looking to do two papers. Thank you for your feedback.

Hi Joe, thank you for your feedback!

I didn't know about the ATCC!, Thank you for this tip! I explained it better on the other answers. As you can see I'm looking towards to do a biological validation, but on another close related species. It's because the public data was so complete, that i got excited and did some deep discussion through differential expression analysis, however this was not the main objective of the "final" paper which is about the pipeline/algorithm per se. so I thought about do another paper.