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I asked the guy if it was laminar flow and he said it was UV hood to
prevent cross-contamination for their RNA work. The hood was a large
clear chamber able to fit on a normal lab workbench. They have the
wall mounted flow hoods for other jobs like cell culture.
UV in this sense is just to break down the RNA, since its more labile
than DNA anyway. I would think it would have small arm holes to
prevent air currents as much as possible, did it?
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Nathan McCorkle
Rochester Institute of Technology
College of Science, Biotechnology/Bioinformatics
I don't know the exact hood in question, but the UV breaks down
everything, DNA, RNA, Protein, liposomes, acrylics and polycarbonates
(I think) will photo-oxidize and 'craze'.
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Some laminar flow hoods will use UV light to sterilize air internally.
Most of the UV hoods I've worked in either; A.) Had a sash switch so
that arms in/out -> lights off/on or B) had a timer that turned the
lights on for X number of hours after use. IIRC, bacterial spores are
about the only thing you need to worry about in a UV hood.
Sent from my mobile Android device, please excuse any typographical errors.
No, he (and I) mean bacterial... it should be easily googlable
> No, he (and I) mean bacterial... it should be easily googlable
>
I assume this is the endospore (from wikipedia articles). The
Firmicutes form these spores but how common are these type of bacteria
in labs? Could they be brought in from outside? That's why I asked if
it was a typo.
They're use in lab is fairly typical. The "BT" in "BT corn" is
Bacillus thuringiensis. The entire (or nearly) Bacillus genus is spore-
forming. My familiarity with Bacillus thuringiensis is as a model
organism for Bacillus Anthracis, Bacillus subtilus is used for the
same purpose. I'm no environmental monitoring expert, but I feel
confident in saying that unless you're in a clean room, I would assume
that they're (endospores) there, and probably contaminating anything
that isn't sealed and sterilized.
From one of my alma maters:
https://engineering.purdue.edu/CE/Academics/Groups/Environmental/Details/FacultyInfo/EBlatchley/EBlatchley/Links/InactivationBacillusSpores.pdf
Although the firmicutes are the only true endospore formers AFAIK, the
Clostridia also make tough spores that can survive boiling or even brief
pressure cycles, and many fungal spores can likewise outlast punishing
conditions. However, even an endospore will succumb to *enough* UV..
it's just that such excessive exposures are costly and pose a
sunburn/cancer risk to anyone directly exposed. So, dilute H2O2 will do.
Easiest cheap source of dilute H2O2 is "Napisan", a brand name form of
sodium percarbonate. Sodium percarbonate is a salt of hydrogen peroxide,
so you don't have to worry about the shelf life of the H2O2, as you can
dissolve it fresh right before use. You do have washing soda (sodium
carbonate) in this mix as well, so you have to wipe surfaces down after
use or deal with a crusty precipitate, but I think that's a fair
tradeoff for the convenience.
All that said, I've been working with B.subtilis for quite a while now,
and I don't find that the lab strain poses much of a contamination
problem. 25min autoclave cycles will sterilise everything very
efficiently, and the lab strains are even susceptible to boiling; they
form very poor quality spores.
All the best,
Cathal
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www.indiebiotech.com
twitter.com/onetruecathal
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PGP Public Key: http://bit.ly/CathalGKey
Thankfully I now have a control plasmid, and I'll shortly have
antibiotics. If direct comparison of transformation methods isn't enough
to test the plasmid by reference to the control, I can PCR in the
resistance cassette from the control to test further.
And the plasmid *will* be biobrick compatible, along with a bunch of
other design goodies. :) Segregational stability should be one!
On 14/12/11 01:50, Simon Quellen Field wrote:
> I'm interested in your progress with gram positive DIY.
>
> Meredith and I both wanted to play with yogurt cultures, but the
> non-availability
> of BioBrick-type plasmids for gram positive bugs made this difficult for
> DIY.
As I said, my experience with UV was with SPDT-type, sash, or dial
timer switches so that a concerted effort was required to expose
oneself to the UV. The UV was considered more 'last ditch' and 'broad
spectrum' breaking down cells, DNA, RNA, Proteins, toxins, blood
pathogens, etc. If nothing else, it was good for enforcing lab order
and cleanliness, anything that was left out at the end of the night
got a good dose of UV. Kinda like slowly autoclaving all the visible
surfaces in lab every night.