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Transcript
Recombinant DNA Techniques Laboratory Bi 431/531 • • • • • • • Introduction/Syllabus Class Overview Bioluminescent bacteria Micropipetting – Exercise I, part I Aseptic techniques – Exercise I, part II Environmental Isolates – Exercise III Start liquid cultures for Wednesday Introduction/Syllabus • • • • • • Office hours Lab safety Gloves- no gloves in hallway! Quizzes Participation Lab notebooks – Ink, math, up to date, random checks • • • • Lab reports Environmental isolates Grad presentations Handouts/Mol review Bioluminescent Bacteria • Present in many deep sea organisms and in the open ocean • Most belong to genus Photobacterium, some to Vibrio • The lux operon – 5 genes, about 8 kb – Three genes remove Acyl ACP from fatty acid biosynthesis pathway – Two genes code for the α and ß subunits of luciferase Bioluminescent Bacteria • Quorum sensing – Operon is turned on and off by the presence of an autoinducer • acylhomoserine lactone, used by many microbes – Expression only occurs at high cell density ~107cells/ml Projects • Cloning the Lux operon – Grow and purify DNA from cultured bioluminescent organisms – Remove the lux operon with restriction endonucleases or PCR from genome – Ligate into plasmid – Transform into E.coli – Screen for bioluminescent E. coli • Isolation of “wild” bioluminescent bacteria – Use sea samples to grow and isolate bacteria – Create a pure stock and cryogenically freeze – Amplify and sequence part of a lux gene to identify the organism Exercise I - Micropipetting • Pipetter safety – read and always follow cautionary notes on page 3 • Tubes A & B – Combine the appropriate volumes of 10X buffer, DNA, H2O and Enzyme spin check final volume (should be 10ul) • Tubes C-F – Combine same components along with Reagent A spin check final volume (should 100ul for C&D, 1000ul for E&F) Aseptic techniques – Exercise I, part II • Streaking agar plates – 4 different bacterial cultures will be streaked: • • • • E.coli DH5α – both LB and LB Amp plates E.coli DH5α (pGEM-3Zf[+]) – both LB and LB Amp plates Photobacterium leognathi – PB plates Vibrio fisheri – PB plates – Streaking DEMO • Broth culture inoculations • E.coli DH5α (pUWL500 or pUWL506)– LB Amp • E.coli DH5α (pGEM-3Zf[+]) – LB Amp – Add 40 ul of Amp to LB tubes) • Photobacterium leognathi – LBS • Vibrio fisheri – LBS Environmental Isolates • Goal is to sequence the lux genes in environmentally isolated bacteria • Each person will isolate their own strain • Procedure is Ex III in Winfrey et al. • PB plates will be used instead of LBS • Each person will streak two PB plates from the provided sea creature Checklist • Streaking agar plates • • • • E.coli DH5α – both LB and LB Amp plates E.coli DH5α (pGEM-3Zf[+]) – both LB and LB Amp plates Photobacterium leognathi – PB plates Vibrio fisheri – PB plates • Broth culture inoculations • • • • 2 E.coli DH5α (pGEM-3Zf[+]) – LB Amp Broth (for Wednesday Plasmid Prep) Photobacterium leognathi – LBS Vibrio fisheri – LBS 2 sea creature PB plate innoculations – INCUBATIONS • E.coli strains – 37° • Biolumiescent strains – room temperature • FOR THURSDAY: • • • • Read Molecular review worksheet Answer/hand in questions (this is this weeks quiz) Read Ex 6 Plasmid Prep (just the intro) Read GeneJET™ Plasmid Miniprep Kit instructions (this is what we will use) Recombinant DNA Techniques Laboratory Bi 431/531 • Exercise 6 –Purification of Plasmid DNA with GeneJET™ Plasmid Miniprep Kit Large-Scale purification of Plasmid DNA • Plasmid purification procedures take advantage of two differences between chromosomal and plasmid DNA: – Bacterial chromosomes are much larger than plasmids – Unlike chromosomal DNA, plasmids are not easily sheared and the two strands are physically linked together purification of Plasmid DNA The mini column Large-Scale purification of Plasmid DNA • The DNA purification kit will be used • See handout for procedure details • Use of centrifuge – Centrifuge safety – Balancing – Keeping track of pellets • Store plasmid stocks in the appropriate box in the student freezer YOU WILL NEED THESE LATER!!!!
