Today I made it to the bench, to do plasmid preps to check that some gift plasmids had the expected structure. I needed to check this before freezing stocks of them in our lab strain collection. The plasmids contain fusions of E. coli CRP-S promoters to the E. coli lacZYA genes. I'll be using them as reporters to test my attempts to induce expression of the E. coli sxy gene. The genes are hofM (the E. coli homolog of H. influenzae's comA) and ppdA (the E. coli homolog of H. influenzae's pilB)
So I did minipreps using our nice Sigma kit, and digested the plasmids with a pair of enzymes that would give one of two patterns. I didn't know which of three restriction sites the inserts were in, so I could only predict two possible patterns from my digests (either one 11kb fragment, one 1.2kb fragment and tiny fragments of either ~300 or ~600 (hofM or ppdA); or one 11kb fragment and fragments of ~1.5kb and 1.8kb (hofM or ppdA).
But for the first time in my research career, I absentmindedly plugged the gel box electrodes in backwards - black cable into red connection and red into black. When I went back to check 25 minutes later, the tracking dye was running backwards out the top end of the gel. Rather than starting over, I just reversed the electrodes and let it run back the way it was supposed to go for a couple of hours, hoping that some information would be usable. Much to my surprise, the gel turned out great (the migration process must be perfectly reversible even though the DNA travelled twice through the wells). If the inserts had given the two tiny fragments they would have been lost during the backwards excursion, but luckily the cloning had generated the 1.5 and 1.8kb fragments instead.
- Home
- Angry by Choice
- Catalogue of Organisms
- Chinleana
- Doc Madhattan
- Games with Words
- Genomics, Medicine, and Pseudoscience
- History of Geology
- Moss Plants and More
- Pleiotropy
- Plektix
- RRResearch
- Skeptic Wonder
- The Culture of Chemistry
- The Curious Wavefunction
- The Phytophactor
- The View from a Microbiologist
- Variety of Life
Field of Science
-
-
-
Political pollsters are pretending they know what's happening. They don't.5 weeks ago in Genomics, Medicine, and Pseudoscience
-
-
Course Corrections6 months ago in Angry by Choice
-
-
The Site is Dead, Long Live the Site2 years ago in Catalogue of Organisms
-
The Site is Dead, Long Live the Site2 years ago in Variety of Life
-
Does mathematics carry human biases?4 years ago in PLEKTIX
-
-
-
-
A New Placodont from the Late Triassic of China5 years ago in Chinleana
-
Posted: July 22, 2018 at 03:03PM6 years ago in Field Notes
-
Bryophyte Herbarium Survey7 years ago in Moss Plants and More
-
Harnessing innate immunity to cure HIV8 years ago in Rule of 6ix
-
WE MOVED!8 years ago in Games with Words
-
-
-
-
post doc job opportunity on ribosome biochemistry!9 years ago in Protein Evolution and Other Musings
-
Growing the kidney: re-blogged from Science Bitez9 years ago in The View from a Microbiologist
-
Blogging Microbes- Communicating Microbiology to Netizens10 years ago in Memoirs of a Defective Brain
-
-
-
The Lure of the Obscure? Guest Post by Frank Stahl12 years ago in Sex, Genes & Evolution
-
-
Lab Rat Moving House13 years ago in Life of a Lab Rat
-
Goodbye FoS, thanks for all the laughs13 years ago in Disease Prone
-
-
Slideshow of NASA's Stardust-NExT Mission Comet Tempel 1 Flyby13 years ago in The Large Picture Blog
-
in The Biology Files
Not your typical science blog, but an 'open science' research blog. Watch me fumbling my way towards understanding how and why bacteria take up DNA, and getting distracted by other cool questions.
1 comment:
Markup Key:
- <b>bold</b> = bold
- <i>italic</i> = italic
- <a href="http://www.fieldofscience.com/">FoS</a> = FoS
Subscribe to:
Post Comments (Atom)
Ah, retro-phoresis. I made the same mistake in the last few months of my Ph.D work, which of course is the perfect time for such mistakes ;-) .
ReplyDelete