Ligation Optimization
In order to serve as the template for rolling circle amplification (RCA) in nanoclew synthesis, single-stranded linear DNA must be processed to form a circular template-primer complex.
To synthesize this complex, we first closed the linear template into a loop by annealing the primer to it, and then sealed the nick in the template. For the latter step, we varied the temperature and incubation time of the ligation step to determine the most efficient method for circular complex synthesis.
Nanoclew Synthesis
Duplex Formation
Introduction
Nanoclew synthesis begins with the formation of a circular template-primer complex, which is used by phi29 DNA Polymerase for the rolling circle amplification (RCA) process. During RCA, the polymerase repetitively amplifies the complex, synthesizing ssDNA that folds into the nanoclew.
The process of circular template-primer complex synthesis begins by annealing the primer to the template to form a loop. This is because the primer is complementary to both ends of the linear template (see Image 1). T4 DNA ligase is used to seal the nick in the loop. According to Bullard and Bowater, nick sealing can be completed by incubating at 37°C for 30 minutes [1]. However, NEB recommends doing ligations at room temperature for one hour [2]. Therefore, we sought to determine the optimal temperature and incubation time for creating the circular template-primer complex, as leftover linear strands compete with the circular templates for enzymatic active sites.
Image 1: Linear (top) and circularized (bottom) nanoclew template with the overhang binding site in yellow, palindromic sequences in orange, and primer binding site in green
Aim
To optimize the synthesis of the circular template-primer complex by varying the temperature and incubation time of the ligation reaction.
Techniques Used
Agarose Gel Electrophoresis
Agarose gel electrophoresis allows for the separation of macromolecules like DNA based on size and provides semi-quantitative data regarding the amount of each fragment in the sample based on the brightness of the bands [3]. For this experiment, it was used to elucidate the optimal conditions for template circularization.
Phenol-Chloroform Extraction
Phenol-chloroform extraction is a liquid-liquid extraction technique for purifying DNA samples. The partitioning of the liquid results in a lower organic phase, an interphase containing proteins, and an upper aqueous phase from which DNA can be isolated [4]. We used this technique to purify our circularized template-primer complexes.
Methodology
Image 2: Visual abstract of ligation optimization process
Template-Primer Annealing
Template and primer (IDT) were diluted to master stocks of 100 µM using pH 7.5 IDTE Buffer. Working stocks of 10 µM of both were then made using Milli-Q water. The template and primer were then combined with T4 ligase buffer (NEB) and diluted with water to the following final concentrations:
Component |
Concentration |
10x T4 Ligase Buffer |
1x |
10 µM Template Stock |
0.6 µM |
10 µM Primer Stock |
1.2 µM |
Template Ligation
Following that, the sample was heated to 95°C for 5 minutes and cooled to room temperature for approximately 2.5 hours, decreasing at a rate of one degree every two minutes. Afterwards, 10 U of T4 ligase (NEB) was added for every microliter of the reaction. The sample was then subjected to one of the treatments listed above.
After the designated incubation time, the sample was heated to 65°C for 10 minutes to deactivate the T4 ligase.
Phenolchloroform Extraction
A volume of phenol:chloroform:isoamyl alcohol (25:24:1) (Thermo Fisher) equal to that of the sample was added and the sample was vortexed for 20 seconds. After centrifuging for five minutes at 16,000 g, the aqueous phase was removed and transferred to another tube.
The following reagents were then added (glycogen was acquired from Thermo Fisher):
Component |
Concentration |
Amount |
Glycogen |
20 µg/µL |
1 µL |
Ammonium acetate |
7.5 M |
0.5x sample volume |
Ethanol |
100% |
2.5x sample volume |
The sample was incubated at -20°C for an hour, and then centrifuged at 4°C for 30 minutes at 16,000 g. The supernatant was removed and the pellet was washed twice with 70% ethanol followed by resuspension by centrifugation at 4°C for 2 minutes at 16,000g. Finally, the pellet was left to air dry for 10 minutes and resuspended in Milli-Q water.
Agarose Gel Electrophoresis
A 2% agarose gel was prepared using Top Vision Agarose (Thermo Fisher) and diluted 10x TBE buffer (Sigma-Aldrich). The samples were mixed with 6x purple loading dye (NEB) and ran at 120V until the dye front was two-thirds of the way down the gel. The gel was then imaged using the MultiImage Light Cabinet and the AlphImager program.
Results
Image 3: Photo of an agarose gel showing the banding patterns made by template-primer complexes that have been subjected to different ligation conditions
As demonstrated by Image 3, while all conditions yielded successfully ligated circular template-primer complexes, incubation for 30 minutes at either temperature resulted in an excess of linear templates. Additionally, the band for the one-hour incubation at room temperature was darker than the band for the one-hour incubation at 37°C, suggesting that more complexes were formed.
Discussion
Incubating samples at room temperature was found to be optimal in minimizing the amount of linear template leftover and maximizing the amount of circularized template-primer complexes (marked by a star in Image 3). Contrary to the findings of Bullard and Bowater, incubating at 37°C for 30 minutes was not sufficient to completely seal all nicks in the templates. This is possibly due to the template being circular, whereas their strands were linear, which may contribute to steric hindrance that prohibits rapid ligation.
References
1. Bullard, D.R. & Bowater, R.P. (2006). Direct comparison of nick-joining activity of the nucleic acid ligases from bacteriophage T4. Biochem J., 398(Pt 1), 135-144.
2. Biolabs, N. E. (n.d.). Ligation Protocol with T4 DNA Ligase (M0202). Retrieved from https://international.neb.com/Protocols/0001/01/01/dna-ligation-with-t4-dna-ligase-m0202.
3. Agarose Gel Electrophoresis. (n.d.). Retrieved from https://www.addgene.org/protocols/gel-electrophoresis/.
4. Sambrook, J. & Russell D.W. (2006). Purification of nucleic acids by extraction with phenol:chloroform. CSH Protoc., 2006(1). doi: 10.1101/pdb.prot4455.
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