Thermostable Terminal deoxynucleotidyl Transferase (ThTdT)

Thermostable Terminal Deoxynucleotidyl Transferase (ThTdT) is a mutated template-independent DNA polymerase originating from Bos taurus. This protein coding basic part performs template-free nucleotide triphosphate (dNTP) addition at the 3’ end, requiring a starting primer. Recombinantly isolated from DH5α E. coli, the enzyme is a thermostable variant of its wild type counterpart enabling an increased working temperature range of 37°C to 55°C (as tested) and requires a divalent cation such as Co²⁺ to increase its 3’-extension efficiency (used in characterization experiments).

Sequence and Features

Assembly Compatibility:

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Clickable Table of Contents

1. Usage and Biology

1.1 Terminal deoxynucleotidyl Transferase (TdT)

1.1.1 Wild type TdT (WT TdT) Overview

What is the WT TdT enzyme and what is its function?

fig1.1 — Fig. 1.1: Terminal deoxynucleotidyl Transferase (TdT) catalyzes the addition of nucleotide triphosphates (dNTPs) to the 3’-termini of single stranded DNA (ssDNA).

Terminal deoxynucleotidyl transferase (TdT) is a uniquely template-independent DNA polymerase (Ashley et al., 2023). Chemically, TdT elongates the free 3’-hydroxyl termini of DNA molecules, typically a primer, using deoxyribonucleotide triphosphates (dNTPs) as substrates, forming inorganic pyrophosphate (PP_i) as a by-product. It plays a key role in diversifying the human cell receptor portfolio of T- and B- cell receptors by V(D)J recombination. This is achieved by adding non-templated nucleotides between the V, D, J exons (Motea & Berdis, 2010).

What organism does WT TdT originate from?

TdT belongs to the X family of polymerases, responsible for DNA repair in mammals (Hoitsma et al., 2020). It was one of the first mammalian polymerases to be identified, originally extracted from the cow thymus in 1960 (Bollum, 1960). Therefore, the wild type TdT (WT TdT) we use for our project (see below), nuCloud, comes from cows. Similarly, the thermostable TdT (ThTdT) used is also of bovine origin (Chua et al., 2020).

What is the chemical catalytic reactivity of WT TdT?

As a transferase (Enzyme Commission EC 2.7.7.31), TdT catalyzes the following reaction:

Oligonucleotide_n + dNTP → Oligonucleotide_n+1 + PP_i

How is WT TdT's reactivity modulated?

WT TdT has optimal activity at approximately 37ºC, and it inactivates at 40ºC (Chua et al., 2020; Boulé et al., 2000). TdT is also a metalloenzyme, where either one of Mg²⁺ or Mn²⁺ is required for catalytic activity (Pandey et al., 1987). Other divalent transition metal cations, such as Co²⁺ and Zn²⁺ are known to enhance its transferase activity, especially with dCTP and dTTP (Grosse et al., 1993; Ratliff, 1981).

1.1.2 Thermostable TdT (ThTdT) Overview

What are the limitations of WT TdT? Why do they matter?

As TdT adds nucleotides to the growing ssDNA strand, the increasing sequence length reduces the energetic stability of the ssDNA (Bochman et al., 2012). This causes the oligonucleotide strand to fold back on itself, forming undesired secondary structures. These secondary structures, in particular, have been shown to reduce the efficiency of TdT activity (Barthel et al., 2020).

How can Thermostable TdT (ThTdT) help?

fig1.2 — Fig. 1.2: Comparison of thermostability and function between WT TdT and ThTdT between 37ºC and elevated temperatures.

To address the incumbrance of secondary structures, increasing the reaction temperature is a preferable approach, as it weakens intramolecular hydrogen bonds and prevents the formation of secondary structures (Barthel et al., 2020). To facilitate the reaction at elevated temperatures, we engineered a more thermostable version of TdT using synthetic biology techniques, which we named thermostable TdT (ThTdT). ThTdT is designed to retain functionality at elevated temperatures, enabling reliable long oligonucleotide production without secondary structure interference. According to Barthel et al. (2020), ThTdT was shown to function up to 47ºC, 10 ºC higher than the unmodified TdT.

How did the mutations change the structure of TdT relative to wild type?

fig1.3 — Fig. 1.3: Three-dimensional models of terminal deoxynucleotidyl transferases (TdT) as ternary complexes with ssDNA (dA)₅dT (as cartoon), 2’,3’-dideoxythymidine 5’-triphosphate (green sticks), Mg²⁺ ion (green sphere) and Na⁺ ion (red sphere). A. WT TdT (white), with X-ray structure adapted from PDBID 4I27. B. ThTdT (red) with the mutated sequence. C. Superposition of WT TdT (white) and ThTdT (red) at the loop adjacent to the active site, where residues 339 and 340 were depicted as sticks. In particular, the mutant ThTdT N_ε atom in K339 was proposed to hydrogen bond with the peptide backbone of G337, with a measured bond length of 3.3 Å.

Video. 1.1: Overall three-dimensional structural comparison of WT TdT (grey) versus ThTdT (red).

Video. 1.2: Three-dimensional ThTdT structure highlighting location of the mutant ThTdT N_ε atom in K339 forming the hydrogen bond with G337.

ThTdT carries 11 point mutations relative to the wildtype, where 9 are outside of the substrate binding pocket. Within the binding pocket, two substitution mutations were found in the active site, M339K and T340I. Notably, M339K was predict to afford a new hydrogen bond with G337, which may confer higher thermostability alongside with other mutations. While this conformer requires further validation, other possible stabilization modes, such as solvation, may be plausible in the improved thermostability.

1.2 Current Applications of TdT

Beyond applications in DNA data storage, TdT is used in other areas of research and industry:

Research
- Molecular probe generation
  - Using chemically modified nucleotide triphosphates, such as fluorophore and digoxigenin conjugates, antisense based molecular probes were synthesized by TdT to generate highly specific targeting agents for biological imaging and disease etiology studies (Lu et al., 2022).
- Polynucleotide synthesis
  - Standard DNA synthesis uses phosphoramidite chemistry and require punctiliously anhydrous and volatile organic reagents, as opposed to chemoenzymatic synthesis that occurs in aqueously buffered salts (Barthel et. al, 2020). Pivoting to enzymatic synthesis via optimized use of polymerases, like TdT, provides scope for cheaper and greener polynucleotide synthesis.
- DNA nanotechnology
  - TdT has been demonstrated to aid in the assembly of DNA nanostructures such as hydrogels. DNA hydrogels require DNA building blocks, which can be enzymatically synthesized using TdT (Xiang et. al, 2016). TdT can be used to add complementary DNA tails to the building blocks which allows for hybridization between the blocks and formation of the gel structure.
- Biosensors
  - TdT has been applied to develop new biosensing platforms as well as to amplify the output of biosensors. TdT’s ability to add multiple nucleotides of the same base can be used to generate poly dA tails. These polynucleotide tails have been used for sensitive detection of the activity of various molecules such as uracil-DNA glycosylase (Du et. al, 2021).
Industry
- Companies have also started adopting the use of TdT in developing new products to perform DNA synthesis. DNAScript launched the first benchtop DNA printer, SYNTAX, run on enzymatic DNA synthesis technology, and TdT plays a critical role in the elongation of DNA in the workflow (Grinstein, 2023).

1.3 Usage with nuCloud

1.3.1 About nuCloud

What is the purpose of the project?

fig1.4 — Fig. 1.4: ThTdT as the centerpiece data-writing basic part of UBC iGEM 2024’s biomanufacturing data storage technology, nuCloud.

Our project, nuCloud, aims to address the need for a sustainable, more energy-efficient data storage medium compared to current magnetic and optical data storage options. One direction through which we tackle this issue is by developing an enzymatic DNA synthesis platform that can elongate single-stranded DNA (ssDNA) in a template-independent manner. The synthesized ssDNA strand will then be converted to a more stable, double-stranded DNA (dsDNA) and can be inserted into a plasmid for long-term data storage. We will leverage TdT’s ability to elongate DNA in a template-independent manner to perform enzymatic synthesis of the original ssDNA strands that are needed for data storage.

1.3.2 ThTdT in nuCloud

In nuCloud, ThTdT enables synthesis of custom nucleotide sequences encoding data for storage efficiently and sustainably. Even with the efficiency gains of ThTdT, template-free DNA synthesis remains a highly repetitive process, adding only one nucleotide per reaction cycle. To overcome this, we leverage microfluidic platforms to automate the synthesis process, and on top of that, minimize the amount of ThTdT and reagents used.

Liquid Phase Synthesis (LPS)

Prior to solid-phase DNA synthesis, where the primer sequence is immobilized to a glass slide, we tested our ThTdT in a conventional liquid-phase system to verify its ability to add nucleotides to the primer. Liquid-phase synthesis refers that all components. - the ThTdT enzyme, deoxyribonucleotide triphosphates (dNTPs), primer, and Co²⁺ - are in solution. The simple setup also allowed us to perform characterization tests on ThTdT over a range of temperatures and concentrations.

Solid-phase synthesis (SPS)

Solid-phase DNA synthesis is the strategy that immobilizes the primer to be extended onto a solid support. Unlike LPS, an immobilized primer means that after a nucleotide has been added, the liquid phase can be washed away and a new solution containing the next nucleotide can be added, akin to solid phase oligonucleotide synthesis without the harmful chemicals. This strategy allows us to precisely control the bases added per cycle, allowing us to synthesize any DNA sequence suitable for storing data. We designed and produced reusable microfluidic chips to facilitate solid-phase enzymatic DNA synthesis with our ThTdT, enabling resource-saving small reaction volumes, and an automated workflow.

2. Characterization of ThTdT

2.1 Designing the ThTdT Gene Fragment

To generate the Thermostable TdT gene fragment (ThTdT), the DNA sequence from Chua et al. (2020) was used to combine with an N-terminal His₆, thrombin cleavage site, and SUMO tag in silico. (Fig 2.1).

fig2.1 — Fig. 2.1: *ThTdT* gBlock: His₆ Tag, Thrombin site, SUMO tag, *ThTdT* gene sequence. 1515bp.

The in silico result was synthesized via the IDT gBlock synthesis service.

2.2 Cloning of ThTdT

The pET-28b plasmid backbone was obtained from Novagen. To remove multiple cloning site (MCS) and undesirably positioned His₆-tag from pET-28b, inverse PCR was performed on pET-28b plasmid. A 30 bp overhang in the ThTdT gene fragment was included in preparation for Gibson assembly (Figure 2.2).

fig2.2 — Fig. 2.2: Diagnostic PCR results using agarose electrophoresis. I1+I2: Amplicon product from pET-28b by inverse PCR using primers P5, P6, expected product size 5198 bp, A1+A2: Amplicon product of *ThTdT* via PCR using primers P3, P4, expected product size 1545 bp. Ladder: 1 kb DNA size ladder, 10% Agarose gel, 45 min, 120 V, SYBR Safe. P3: TTCCTTTCGGGCTTTGTTAGCAGCCGGATCCTAAGCATTTCTTTCCCATGGTTCA, P4: ATTTTGTTTAACTTTAAGAAGGAGATATACATGGGCAGCAGCCATCATC, P5: ATGGCTGCTGCCCATGTATATCTCCTTCTTAAAGTTAAACA, P6: GAAAGAAATGCTTAGGATCCGGCTGCTAACAAAGC.

fig2.3 — Fig. 2.3: pET-28b(+) plasmid map with *ThTdT* insert.

Using Gibson assembly, ThTdT was ligated with the modified pET-28b plasmid. The product was then transformed into chemically competent DH5α E. coli (Figure 2.4). Successful ligation and transformation were indicated via colony growth on an LB-Kanamycin (50 µg/mL) plate. Further validation was completed by colony PCR (Figure 2.5) and whole plasmid sequencing by Plasmidsaurus (Figure 2.6).

fig2.4 — Fig. 2.4: LB-Kanamycin (50 µg/ml) plate, plated with DH5a Gibson assembly product transformed cells.

fig2.5 — Fig. 2.5: Colony PCR confirmation of Gibson assembly and from LB-Kanamycin plate transformants using primers P3 and P4. 1 kb DNA size ladder. 10% Agarose gel, 45 min, 120 V, SYBR Safe. Product size of ~1500 bp. Ladder: 1 kb DNA size ladder, C1: Colony 1, C2: Colony 2, C3: Colony 3, C4: Colony 4, R1: *ThTdT* gBlock. P3:TTCCTTTCGGGCTTTGTTAGCAGCCGGATCCTAAGCATTTCTTTCCCATGGTTCA, P4:ATTTTGTTTAACTTTAAGAAGGAGATATACATGGGCAGCAGCCATCATC.

fig2.6 — Fig. 2.6: Sequencing result of pET-28b(+)-*ThTdT* completed by Plasmidsaurus. Out of 6716 bases sequenced, in the *ThTdT* gBlock region, 2 silent mutations were detected: T4194G, C4629T.

2.3 Purification of ThTdT

Plasmids were extracted from DH5α and transformed into BL21 (DE3) for ThTdT protein expression (Fig 2.7). ThTdT expression was induced with IPTG in transformed BL21, followed by mechanical lysis to obtain crude cell lysate. Isolation of ThTdT was completed with Ni-NTA magnetic beads (New England Biolabs, NEB). Fractions containing ThTdT was confirmed via SDS-PAGE (Fig 2.8). To remove the excess imidazole from the protein elution buffer, the combined ThTdT-containing fractions were purified using Amicon® Ultra Centrifugal Filter system to concentrate the samples. For long term storage, the purified protein was formulated in NEB storage buffer in-house (50 mM potassium phosphate, 100 mM NaCl, 1.43 mM β-mercaptoethanol, 50% Glycerol, 0.1% Triton® X-100, pH 7.3 @ 25°C) that was recreated in-house. The storage buffer was also supplemented with 100 µM 2,2’-bipyridyl to remove residual contaminating Ni²⁺ that was carried over from purification.

fig2.8 — Fig. 2.8: SDS-PAGE of ThTdT isolated after magnetic beads purification. 120 V, 1.5 h, Coomassie Blue staining. MW: Molecular Ladder, L: Cell lysate, E1: elution fraction 1, E2: elution fraction 2.

2.4 Proof of Function: Liquid Phase Synthesis (LPS)

2.4.1 Benchmark Establishment using WT TdT (LPS)

Using the in-house ThTdT, 3’-elongation activity to Cy5-labeled primer P1 was observed using all four canonical nucleotide triphosphates at temperatures above 40ºC. This was chosen because it was the upper temperature limit for WT TdT to retain its function (Chua et al., 2020). In order to test this hypothesis, a liquid phase synthesis (LPS) system was devised to validate nucleotide addition. Firstly, WT TdT purchased from NEB was studied to develop a standard assaying condition for all four nucleotide triphosphates (Figure 2.9).

fig2.9 — Fig. 2.9: Nucleotide addition to primer using WT TdT with varying dNTP concentration. Primer P1 /5Biosg/ ATT CGrA TCA /iCy5/CTA GCA TAC TAT CAT TCG GGG. [Primer] = 100 nM. Reaction Time = 30 min. Temperature = 37ºC. Denaturing Urea PAGE, 20%, 400 V, 30 min.

This supports the claim that our system was successful in catalyzing nucleotide addition and this condition could be used as a benchmark against our in-house ThTdT. This also validated that denaturing PAGE following fluorescent detection on a Typhoon biomolecular scanner was an efficacious workflow to visualize the results.

2.4.2 Functional Validation of ThTdT (LPS)

With a benchmark assay available, the ability for our in-house ThTdT to incorporate nucleotide triphosphates to an oligonucleotide was studied. Gratifyingly, purified ThTdT stored in a modified NEB storage buffer was able to incorporate nucleotides in primer 2.

fig2.10 — Fig. 2.10: 3’-extension by wild type terminal deoxynucleotidyl transferase (WT TdT) and thermostable terminal deoxynucleotidyl transferase (ThTdT) using primer P2 /56FAM/AGCCTGTTGTGAGCCTCCTAAC at 37ºC for 15 min. [Primer P2] = 100nM, [CoCl2] = 250 µM, [dNTP] = 1 µM. 20% D-PAGE, 30 min, 400V. Imaged using Cy3 setting.

2.5 Proof of Function: Solid Phase Synthesis (SPS)

2.5.1 Oligonucleotide Functionalization on Glass (SPS)

Encouraged by the success in LPS, the focus turned to solid phase synthesis (SPS). SPS refers to the strategy where an immobilized, yet cleavable, oligonucleotide to be 3’-extended using any TdT. The reason why a base-cleavable linker was included was to allow rapid cleavage of the ThTdT-treated ssDNA for denaturing PAGE analysis. To encapsulate these notions, P1 was designed for this purpose.

fig2.11 — Fig. 2.11: Functional features of P1/5Biosg/ATTCGrATCA/iCy5/CTAGCATACTATCATTCGGGG. The 5’-terminus is functionalized with biotin. All sugar backbone consists of deoxyriboses, except at the ribose back cleavage site (red arrow) where the ribose linkage is base-labile. The fluorophore of choice in P1 is Cy5, which is used for fluorescent detection. The free 3’-terminus allows TdT to add nucleotide triphosphates to extend to the right.

A few steps were applied to a microscope glass slide in order to receive the primer for functionalization (Fig. 2.12). The slides were first silanized using Piranha solution (25% v/v H₂O₂, 75% v/v H₂SO₄), followed by introduction of 3-aminopropytriethyoxysilane (APTES) to install free amine groups. Following standard amide coupling conditions with N-hydroxysuccinimide esters of PEGylated acids and biotin conjugates (99:1 mole ratio), a biotinylated glass surface was afforded. Since streptavidin is a potent binder of biotin, for the scope of this work, it serves as a natural linker between two biotinylated moieties, namely the biotinylated glass slide, and the biotinylated P1.

2.5.2 Functional Validation of ThTdT (SPS)

Via fluorescent imaging, Figure 2.13 demonstrated that P1 was functionalized onto glass. ThTdT, along with other cofactors and substrates, were directly applied to the oligonucleotide-immobilized glass as a 10 µL droplet.

fig2.13 — Fig. 2.13: Fluorescence imaging of microscope glass slide with Cy5 fluorescently labeled primer P1 immobilized at selected locations, prior to (A) and after (B) ThTdT extension. P1 /5Biosg/ATTCGrATCA/iCy5/CTAGCATACTATCATTCGGGG.

The reaction droplets were removed by pipetting, followed by aqueous washes to remove residual reactants. Gel loading buffer, supplemented with 0.1 M NaOH, was loaded directly on top of the reacted glass patches to quench the reaction and to cleave and denature the ssDNA of interest for separation on denaturing PAGE.

fig2.14 — Fig. 2.14: 3’-extension by ThTdT on using primer P1 /5Biosg/ATTCGrATCA/iCy5/CTAGCATACTATCATTCGGGG immobilized on microscope glass slide at 37ºC for 30 min. Lanes 1, 2, and 3 contains 10 fmol, 1 fmol, and 100 amol P1. Lane 4 contains reaction crude from SPS, reacted in [CoCl₂] = 250 µM, [dTTP] = 10 µM. 20% D-PAGE, 30 min, 400V. Imaged using Cy5 setting.

This SPS system demonstrated promising preliminary efficacy in incorporating dTTP to P1, as demonstrated by Figure 2.14, where the SPS-treated sample, following cleavage in NaOH, had more mass than the primer-only negative control.

3. References

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