Week 6 HW — Genetic Circuits Part 1

Week 6 — DNA Assembly

1. Phusion High-Fidelity PCR Master Mix components

The Phusion High-Fidelity PCR Master Mix contains several key components:

  • Phusion DNA Polymerase
    A high-fidelity enzyme that synthesizes DNA with very low error rates.

  • dNTPs (deoxynucleotide triphosphates)
    The building blocks used to construct new DNA strands.

  • Buffer system
    Maintains optimal pH and salt conditions for enzyme activity.

  • Mg²⁺ ions
    Essential cofactor for DNA polymerase function.

  • Stabilizers and additives
    Help improve enzyme performance and reaction efficiency.

The purpose of this mix is to ensure accurate and efficient DNA amplification, especially important for cloning and assembly workflows.

2. Factors determining primer annealing temperature

Primer annealing temperature depends on several factors:

  • Primer length
  • GC content (higher GC → higher melting temperature)
  • Sequence composition
  • Salt concentration in the buffer
  • Primer complementarity

In practice, annealing temperature is typically set slightly below the melting temperature (Tm) of the primers to ensure specific binding.

3. PCR vs Restriction Digest

Both PCR and restriction digestion can produce linear DNA fragments, but they differ significantly:

PCR

  • Amplifies DNA using primers
  • Can create custom sequences
  • Allows addition of overlaps for cloning
  • More flexible but requires careful primer design

Restriction Digest

  • Uses enzymes to cut DNA at specific sequences
  • Produces predictable fragments
  • Limited by availability of restriction sites

Comparison

MethodAdvantageLimitation
PCRHighly customizableRequires design and optimization
Restriction DigestSimple and reliableDepends on existing cut sites

PCR is preferable when designing new constructs, while restriction digest is useful when working with known plasmids.

4. Preparing DNA for Gibson Assembly

To ensure DNA fragments are compatible with Gibson Assembly:

  • Fragments must have overlapping ends (typically 20–40 bp)
  • Overlaps must be complementary
  • PCR primers are often designed to include these overlaps
  • DNA must be clean and properly amplified

This allows the Gibson Assembly enzymes to seamlessly join fragments.

5. DNA transformation into E. coli

Plasmid DNA enters E. coli through:

  • Heat shock transformation
    Cells are briefly exposed to high temperature, creating temporary pores in the membrane.

  • Electroporation
    An electric pulse creates openings in the cell membrane.

Once inside, the plasmid is replicated by the bacterial machinery.

6. Alternative Assembly Method — Golden Gate Assembly

Golden Gate Assembly is a DNA assembly method that uses Type IIS restriction enzymes and DNA ligase.

Unlike traditional restriction enzymes, Type IIS enzymes cut DNA outside of their recognition site, allowing the creation of custom overhangs.

In this method:

  1. DNA fragments are designed with specific overhangs
  2. Restriction enzymes cut the DNA
  3. Compatible overhangs anneal
  4. DNA ligase joins the fragments

Because cutting and ligation happen in the same reaction, Golden Gate Assembly allows efficient and ordered assembly of multiple DNA fragments in a single step.

This makes it highly useful for building complex genetic constructs.

7. Assembly Method Explanation (5–7 sentences)

Golden Gate Assembly is a one-pot DNA assembly technique that enables the precise joining of multiple DNA fragments. It relies on Type IIS restriction enzymes, which cut outside their recognition sites, generating user-defined overhangs. These overhangs are designed to be unique and complementary, ensuring correct fragment order. During the reaction, restriction enzymes and ligase work simultaneously: fragments are cut and immediately ligated. Because the recognition sites are removed during assembly, the final construct is stable and cannot be re-cut. This makes the process highly efficient and directional. As a result, Golden Gate Assembly is widely used in synthetic biology for building modular genetic systems.

Design Reflection

DNA assembly can be understood as a form of modular design, where genetic elements behave like components that can be recombined, layered, and reorganized.

Methods such as Gibson and Golden Gate resemble different design strategies:

  • Gibson Assembly allows flexible and seamless connections
  • Golden Gate enables structured, rule-based assembly

This parallels architectural systems where materials and components are combined either freely or within strict modular constraints.

Note on Sources

The concepts described in this section are primarily based on the lecture, recitation, and lab protocol materials from this week.

Rather than reproducing the protocol directly, I interpreted these workflows through a design-oriented lens, organizing them as modular systems and comparing different assembly strategies.

This approach helped me better understand DNA assembly not only as a technical process, but also as a form of structured design.