Hi!,
Did you grow your E.coli in the presence of an antibiotic and select for plasmid containing cells? How do you know what you are seeing is plasmid? Can it be partially digested RNA? If it's plasmid DNA, yes you will sequence it. If it's as much as your gDNA, you should expect that half of the reads would be plasmid reads?

You can also gel purify your genomic DNA and make a library. You can digest agarose by β-Agarase. I have not tried it myself buy one of my colleague do it all the time for genomic DNA extraction from agarose. NEB has a library prep that allows you to make libraries as little as 1-5 ng input DNA. It's called "NEBNext Ultra DNA Library Prep Kit for Illumina". By the way, I believe Qubit dye cannot bind supercoiled DNA and you need to linearize it. Hope this helps.

Have you isolated those bands and sequenced them, to determine what they are?

Thank you for your answers!
I have news: I repreped my gDNA since covaris shearing didn't work as expected. In the new DNA prep I did a RNaseA treatment and now both bands are gone. I assume that the bands weren't plasmid bands at all but were 23s & 16s rRNAs. My band patterns are very similar to those in A (not my image!):



I would love to upload my gel pictures but my program is very strict about plagiarism and I assume they will start picture comparison next ...

Hi rnaeye!
Yes one of the strains grew on AB but didn't show the two bands. I just assumed that it was plasmids displaying the bands. I think you are right about your RNA assumption since I didn't RNaseA treat my samples. I kind of assumed that I would work dirty enough to get rid of them .
And I Qubit my sheared DNA and PicoGreen my gDNA.

Funny thing is that it is possible to MiniPrep plasmids from these strains!

Hi Brian!
No I haven't done that yet but the plasmid DNA is preped now.

So if the bands are RNA my genomic DNA should be fine I guess. Now I have to rephrase my question: Is it possible to mix in my plasmids in the sequencing run? Should I give them individual indices or rather mix them to the gDNA of the strain of origin? I think giving them individual indices will be the better solution for the subsequent genome assembly?

Thanks again!
Illnoobina

If I had gDNA and plasmid DNA preps separately, I would barcode them and sequence them on the same flow cell instead of mixing them without barcode.

That's what I meant by indivdual indices. So I build a library from each plasmid and gDNA and pool them for sequencing.

How would you pool the libraries? Let's assume the E. Coli genome has a size of roughly 5Mb and my plasmid has an estimated 5kb. So I would concentrate my gDNA 1000x in the library pool and the plasmids 1x?

Yes, you are right. If your goal is to get the same amount of coverage for each genome, you should put 1000x less plasmid DNA since it's smaller.