Week 1: Fragmenting DNA w/ RE
Week 2: Transformation
Week 3: PCR for Water Contaminants
Gel Electrophoresis
Section 1 & 2 Review
100

Sequences that are read the same forward and backward

Palindromes
100
The specific process where exogenous genetic material is directly taken up and incorporated by a cell through its cell membrane

Transformation

100

This is a lab technique that amplifies small segments of nucleic acids

PCR

100

Biology technique that separates DNA based on size

Gel Electrophoresis

100

These are the differences between + and - controls

+ control: used to show a positive test result

- control: used to show a negative test result

200

These cleave (cut) the backbone of DNA molecules at palindromes

Restriction Enzymes

200
The small circular DNA molecule found in bacteria

Plasmids

200

Used in PCR to break open cells to release their components for DNA isolation

Lysis Buffer

200

Labels used for a size standard for comparing DNA bands

DNA ladder
200

The variety of different viruses that can attack the same cell type refers to

Viral cell specificity

300

A specific place on DNA molecule where a restriction enzyme cuts

Restriction enzyme sites or Restriction sites

300

This gene was transformed into the E. coli MM294

ampr

300

This breaks down proteins that could interfere with amplification, including those around the DNA molecule and within the cell

Proteinase K

300

These are formed on gels by many pieces of DNA that are the same and differing sizes

Bands or Restriction Fragments

300

These are the differences between selective and differential media

Selective: Used to selective for the growth of a particular microorganism, inhibiting the growth of others

Differential: used to differentiate closely related organisms, due to presence of dyes/chemicals in media

400

Where the larger molecules are found in an agarose gel

Towards the top

400

Penicillin (Ampicillin in our lab) kills bacteria by blocking the synthesis of

Peptidoglycan in the cell wall during cell division

400

These were found inside of the PCR pellet

Taq DNA polymerase, dNTPs, MgCl2, and buffer

400

TBE (electrophoresis) buffer is used for these two reasons

Provide ions that carry the current to move DNA bands, separate nucleic acids, and provide a stable pH environment

400

This is used to describe the number of different strains or species of organism that a specific virus can infect

Host cell specificity

500

The type/name of cut restriction enzymes EcoRI and HindIII leave on DNA

Sticky ends

500

The steps that are considered critical to the process of transformation

Initial ice incubation, heat shock, secondary ice incubation, and room temperature incubation

AKA Preincubation, Incubation, Heat shock, and Recovery

500

These are the three steps of PCR and what they do

Denaturation: Heat DNA to a high temp that breaks the hydrogen bonds between base pairs

Annealing: Temp is lowered to allow primers to bind to the template strands

Extension: DNA polymerase adds NTs to the 3' end of the primer

500

Loading dye is used in gel electrophoresis for these two reasons

Allow for color DNA visualization and increasing the density of DNA

500

The difference between Gram + and Gram - bacterium

Gram +: stain purple, thick layer of PTG in cell wall

Gram -: stain red/pink, thin layer of PTG in cell wall

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