Week 2 – DNA Read, Write, and Edit

Laboratory Notebook Entry

Metadata

FieldValue
CourseHTGAA
Week2
Dan Wright
TopicDNA Read · Write · Edit

Abstract

This laboratory exercise explored the modern molecular biology workflow: restriction digest simulation, wet-lab electrophoresis, gene design, codon optimization, DNA synthesis preparation, and genome read/write/edit technologies. A developmental transcription factor (MSX-1) was selected, reverse-translated, optimized, and engineered into an expression cassette.

1. Restriction Digest Simulation & Gel Art

Objective

Simulate Lambda DNA restriction digests and generate a gel-art visualization.

Enzymes Used

EcoRI · HindIII · BamHI · KpnI · EcoRV · SacI · SalI

Methods

  • Imported Lambda genome into Benchling
  • Performed multi-enzyme restriction digest
  • Visualized predicted fragment sizes

Result

In-silico restriction digest In-silico restriction digest

Figure 1. Simulated restriction digest of Lambda DNA.

2. Wet Lab Restriction Digest

Objective

Perform physical restriction digestion and electrophoresis following the designed protocol.

3. Gene Design Workflow

3.1 Protein Selection

Target Protein:
MSX-1 (Homeobox protein, Homo sapiens)

Rationale:
MSX-1 regulates developmental gene pathways and limb formation.

3.2 Reverse Translation

Full reverse-translated nucleotide sequence:

atggcccccgccgccgacatgaccagcctgcccctgggcgtgaaggtggaggacagcgcc
ttcggcaagcccgccggcggcggcgccggccaggcccccagcgccgccgccgccaccgcc
gccgccatgggcgccgacgaggagggcgccaagcccaaggtgagccccagcctgctgccc
ttcagcgtggaggccctgatggccgaccacagaaagcccggcgccaaggagagcgccctg
gcccccagcgagggcgtgcaggccgccggcggcagcgcccagcccctgggcgtgcccccc
ggcagcctgggcgcccccgacgcccccagcagccccagacccctgggccacttcagcgtg
ggcggcctgctgaagctgcccgaggacgccctggtgaaggccgagagccccgagaagccc
gagagaaccccctggatgcagagccccagattcagccccccccccgccagaagactgagc
ccccccgcctgcaccctgagaaagcacaagaccaacagaaagcccagaacccccttcacc
accgcccagctgctggccctggagagaaagttcagacagaagcagtacctgagcatcgcc
gagagagccgagttcagcagcagcctgagcctgaccgagacccaggtgaagatctggttc
cagaacagaagagccaaggccaagagactgcaggaggccgagctggagaagctgaagatg
gccgccaagcccatgctgccccccgccgccttcggcctgagcttccccctgggcggcccc
gccgccgtggccgccgccgccggcgccagcctgtacggcgccagcggccccttccagaga
gccgccctgcccgtggcccccgtgggcctgtacaccgcccacgtgggctacagcatgtac
cacctgacc

3.3 Codon Optimization

Full codon-optimized sequence:

ATG GCT CCT GCC GCT GAC ATG ACA TCC CTC CCT CTG GGC GTG AAA GTC GAA GAC TCT GCC TTC GGA AAA CCA GCT GGA GGA GGT GCA GGC CAA GCG CCC TCA GCC GCC GCC GCA ACT GCC GCG GCA ATG GGC GCG GAT GAA GAA GGA GCA AAG CCT AAA GTC TCA CCC TCT TTG CTC CCC TTC TCT GTT GAG GCA CTC ATG GCC GAC CAC AGG AAA CCT GGC GCC AAA GAG TCA GCA CTT GCT CCA TCT GAG GGC GTG CAG GCT GCC GGT GGG TCT GCC CAG CCA CTC GGC GTT CCT CCT GGG TCT CTC GGT GCC CCC GAC GCC CCT AGC TCT CCA CGC CCT CTT GGG CAC TTT AGC GTG GGC GGG CTG CTG AAA CTT CCA GAA GAC GCA CTC GTT AAG GCC GAA AGT CCT GAG AAA CCC GAG CGA ACC CCT TGG ATG CAG TCA CCC AGG TTC TCA CCC CCT CCC GCT AGG AGG CTC TCC CCC CCA GCA TGT ACT CTC CGG AAA CAT AAG ACA AAT AGA AAA CCC CGC ACC CCG TTT ACC ACC GCC CAG CTG CTG GCC CTT GAG AGA AAG TTC CGG CAG AAG CAG TAC CTC TCC ATC GCC GAA CGG GCT GAG TTC TCC TCC TCC TTG TCC CTC ACC GAG ACA CAG GTT AAG ATT TGG TTC CAG AAC CGC CGG GCA AAG GCA AAA CGG CTG CAA GAA GCC GAG CTG GAG AAG CTT AAG ATG GCA GCT AAA CCC ATG CTC CCT CCA GCA GCG TTT GGC CTC AGT TTT CCA CTG GGC GGC CCA GCT GCA GTG GCA GCT GCG GCC GGC GCC TCC CTC TAT GGA GCC TCC GGG CCG TTC CAA CGG GCC GCA CTT CCC GTA GCA CCA GTC GGG TTG TAC ACT GCA CAT GTC GGC TAC AGC ATG TAC CAC CTG ACC

4. Expression Cassette Engineering

Full Expression Cassette Sequence

TTTACGGCTAGCTCAGTCCTAGGTATAGTGCTAGCCATTAAAGAGGAGAAAGGTACCatggcccccgccgccgacatgaccagcctgcccctgggcgtgaaggtggaggacagcgccttcggcaagcccgccggcggcggcgccggccaggcccccagcgccgccgccgccaccgccgccgccatgggcgccgacgaggagggcgccaagcccaaggtgagccccagcctgctgcccttcagcgtggaggccctgatggccgaccacagaaagcccggcgccaaggagagcgccctggcccccagcgagggcgtgcaggccgccggcggcagcgcccagcccctgggcgtgccccccggcagcctgggcgcccccgacgcccccagcagccccagacccctgggccacttcagcgtgggcggcctgctgaagctgcccgaggacgccctggtgaaggccgagagccccgagaagcccgagagaaccccctggatgcagagccccagattcagccccccccccgccagaagactgagcccccccgcctgcaccctgagaaagcacaagaccaacagaaagcccagaacccccttcaccaccgcccagctgctggccctggagagaaagttcagacagaagcagtacctgagcatcgccgagagagccgagttcagcagcagcctgagcctgaccgagacccaggtgaagatctggttccagaacagaagagccaaggccaagagactgcaggaggccgagctggagaagctgaagatggccgccaagcccatgctgccccccgccgccttcggcctgagcttccccctgggcggccccgccgccgtggccgccgccgccggcgccagcctgtacggcgccagcggccccttccagagagccgccctgcccgtggcccccgtgggcctgtacaccgcccacgtgggctacagcatgtaccacctgaccCATCACCATCACCATCATCACTAACCAGGCATCAAATAAAACGAAAGGCTCAGTCGAAAGACTGGGCCTTTCGTTTTATCTGTTGTTTGTCGGTGAACGCTCTCTACTAGAGTCACACTGGCTCACCTTCGGGTGGGCCTTTCTGCG

Annotated Elements

Promoter

TTTACGGCTAGCTCAGTCCTAGGTATAGTGCTAGCCATTAAAG

RBS

AGGAGAAAGG

Spacer

TACC

6×His Tag

CATCACCATCACCATCATCA

Terminator

AGGCATCAAATAAAACGAAAGGCTCAGTCGAAAGACTGGGCCTTTCGTTTTATCTGTTGTTTGTCGGTGAACGCTCTCTACTAGAGTCACACTGGCTCACCTTCGGGTGGGCCTTTCTGCG

Benchling Construct Map

Benchling Construct Benchling Construct

Figure 2. Benchling construct showing CDS, His-tag, and terminator.

5. DNA Read · Write · Edit

5.1 DNA Read

Target genome: Secretariat (racehorse)
Technology: Nanopore sequencing

Workflow:

  1. DNA extraction
  2. Purification
  3. Library preparation
  4. Sequencing
  5. Base calling
  6. Assembly

5.2 DNA Write

Technology: Phosphoramidite synthesis and gene synthesis providers

Steps:

  1. Oligo synthesis
  2. Gibson Assembly
  3. Validation sequencing

Limitations:

  • Fragment size limits
  • Time and cost
  • Assembly complexity

5.3 DNA Edit

Technology: CRISPR knock-in

Mechanism:

  1. Guide RNA design
  2. Cas9 cleavage
  3. Homology-directed repair
  4. Screening

Limitations:

  • Off-target effects
  • Efficiency variability