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Today House Keeping (talks, sequencing) Follow-up on cloning

Published byGarey Fletcher Modified over 8 years ago

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Presentation on theme: "Today House Keeping (talks, sequencing) Follow-up on cloning"— Presentation transcript:

1 Today House Keeping (talks, sequencing) Follow-up on cloning
Transformants? Plasmid extraction Insert check by restriction digest (gel....)

2 Sequencing Many worked, analysis due!
Check and analyze using “Chromas”(freeware) and “Sequencher”, Genecodes provides teaching license for use during the semester! Computers available for sequencher, or use your own; genecodes.com/support/sequencher-server-download

3 PARASITES AND SNAIL BIOLOGY
DNA “identity, possibilities” phylogenetics RNA “intentions” transcriptomics CTAB Trizol gel electrophoresis nanodrop spec Bioanalyzer DNA-free, PCR rDNA/mito TA cloning, B/W screening RT-PCR gel electrophoresis Qiagen plasmid extraction Restriction digests direct sequencing M13 sequencing Sequence ID (BLAST) editing Primer design, walking Phylogenetics GenBank submission 3

4 Work schedule today Each group handout.
“Purelink Quick plasmid extraction" for 4 samples (1.5 ml bacterial culture). EcoRI digest on each sample for insert check on gel. Talk Sequencher

5 Some questions: Did you obtain transformants? What is the composition of plasmids in W and B colonies? How do you recover plasmids? What likely happens in the Purelink Quick plasmid extraction protocol? How can you check for the size of the insert?

6 Do you have the desired insert? How to check Presence, Size of insert

7

8 Gelelectrophoresis Cast gel, load samples, run, take photo……
How long is that going to take?

9 Gelelectrophoresis

10 What to expect? Insert size: Plasmid size: Pattern on gel:
Or digest? Insert size: Plasmid size: Pattern on gel: What primers to use?

11

12 Do you have the desired insert? How to check Presence, Size of insert
Plasmid(linear) insert EcoRI digest of constructs

13 Sequencher?

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