Week 6 HW: Genetic Circuits Part 1

Assignment: DNA Assembly

1. What are some components in the Phusion High-Fidelity PCR Master Mix and what is their purpose?

Phusion DNA Polymerase: This is the “engine.” It’s a highly thermostable enzyme that synthesizes new DNA strands. It’s “High-Fidelity” because it has $3’ \rightarrow 5’$ exonuclease activity (proofreading), making significantly fewer mistakes than standard Taq.
dNTPs (Deoxynucleotide Triphosphates): These are the molecular building blocks (A, T, C, and G) used by the polymerase to construct the new DNA strand.
Buffer (containing $Mg^{2+}$): Maintains the optimal pH for enzymatic activity and provides essential divalent cations. Magnesium ions act as a cofactor for the polymerase, helping it catalyze the phosphodiester bond.
Stabilizers: Often includes detergents or proprietary chemicals to prevent the enzyme from denaturing or sticking to the tube walls during the high-heat cycles.

2. What are some factors that determine primer annealing temperature during PCR?

Primer Length: Longer primers generally require higher temperatures to remain specific.
GC Content: G-C pairs have three hydrogen bonds compared to the two in A-T pairs. Therefore, primers with higher GC content have higher melting temperatures ($T_m$).
Salt Concentration: The concentration of monovalent cations (like $K^+$) in the buffer affects the stability of the DNA duplex.
Primer Concentration: Higher concentrations can slightly shift the kinetics of annealing.
Mismatches: If the primer isn’t a 100% match to the template, the $T_m$ will decrease.

Note: The annealing temperature ($T_a$) is usually chosen to be $3-5^\circ\text{C}$ below the $T_m$ of the primers to balance specificity and yield.

3. Compare and contrast PCR vs. Restriction Enzyme Digests.

Feature	PCR (Polymerase Chain Reaction)	Restriction Enzyme Digest
Mechanism	Enzymatic synthesis of new DNA strands.	Enzymatic “cutting” of existing DNA strands.
Input	Template DNA + Primers + Polymerase.	Plasmid or genomic DNA + Specific Enzymes.
Output	Exponentially amplified linear fragments.	Linearized fragments (no amplification).
Customization	Very high; you define the ends via primers.	Limited to where specific “sites” (e.g., EcoRI) exist.
Accuracy	Risk of point mutations (minimized by Phusion).	Highly accurate sequence retention.

When to use which?

Use PCR when you need to add specific “overhangs” for Gibson assembly or when you have a very small amount of starting material.
Use Restriction Digest when you are moving a large chunk of DNA from a “classic” vector that already contains the necessary sites, or when you want to avoid the risk of PCR-induced mutations in a large gene.

4. How can you ensure that the DNA sequences that you have digested and PCR-ed will be appropriate for Gibson cloning?

For Gibson Assembly to work, your fragments must have homologous overlapping ends (typically 20–40 base pairs).

For PCR: You must design your primers so that the 5’ end of the primer contains a sequence that matches the end of the adjacent fragment.
For Digest: You must ensure the restriction site is positioned such that the resulting linearized DNA shares overlap with the next piece, or use a “Stitch PCR” on the digested fragment to add the necessary overlaps.
Verification: Use a tool like NEB’s Gibson Assembly Designer or Benchling to simulate the “junctions” and confirm the overlaps are in the correct orientation ($5’ \rightarrow 3’$) and have a high enough $T_m$ to stay stable during the reaction.

5. How does the plasmid DNA enter the E. coli cells during transformation?

In the HTGAA lab context, we usually use Chemically Competent cells:

Heat Shock: Cells are kept on ice with DNA, then suddenly moved to $42^\circ\text{C}$.
Pore Formation: This temperature spike creates a pressure imbalance and temporary “pores” or thermal fluctuations in the chemically-weakened cell membrane.
DNA Uptake: The DNA moves through these temporary pores into the cytoplasm.
Recovery: Cells are placed back on ice and then incubated in SOC/LB media at $37^\circ\text{C}$ to “heal” the membrane and begin expressing the antibiotic resistance gene before plating.

6. Describe another assembly method in detail: Golden Gate Assembly.

Golden Gate Assembly relies on Type IIS restriction enzymes (like BsaI or BpiI). Unlike standard enzymes, these cut outside of their recognition sequence, creating custom non-palindromic 4-base overhangs.

Because the recognition site is removed during the cleavage, the reaction is “directional” and “seamless.” This allows for a “one-pot” reaction where digestion and ligation happen simultaneously in the same tube. You can assemble multiple fragments (up to 10+) in a specific order by designing unique 4-bp overlaps for each junction. It is highly efficient and leaves no “scar” sequences if designed correctly.