Difference between revisions of "Team:UChile Biotec/Results"

To validate the utility of JAWS for generating aptazymes sequences from the DNAzyme HRP mimicking and an aptamer for any other molecule, the sequence of an aptamer for AMP was introduced into the program, with the purpose of contrasting the catalytic activity of this aptazyme to the catalytic activity of an aptazyme that has already been characterized and tested in the literature and also by our team last year (APTZ_AMP_P) [1].

The sequence which its free energy difference had the highest value among all of the sequences given by the software was chosen (first sequence of Annex 1, notebook), because this difference consists in the difference of energies between the inactive and active state, so it is the sequence that has the least probability to move from an inactive state to an active state arbitrarily, avoiding false positives.

In addition, since the software delivers sequences with two DNAzymes, one on each flank of the sequence and adjacent to the generated linkers (because the software was designed this way, see Heidelberg 2015 project for more information), the sequences chosen to synthesize and subsequently carry out the enzymatic tests were chosen as delivered by the program (raw) and truncated, with the DNAzyme of the 3 'flank excised based on the configuration of the aptazyme APTZ_AMP_P.

The same procedure was done for DNAzyme HRP mimicking and aptamers specific for saxitoxin (APT_STX) and oxadaic acid (APT_OX) described in the literature [2][3]. All the sequences extracted from the literature and the ones obtained with JAWS are described in Annex 1 (notebook).

2. Testing Sequences

AMP Aptazyme assay:

An experiment was carried out to evaluate if the aptazymes created by JAWS presented a dose-dependent activity for the ligand. Reactions were performed to evaluate the catalytic activity of 3 aptazymes of AMP: the already characterized aptazyme (APTZ_AMP_P) on which there is already evidence of a dose dependence of the ligand, an aptazyme obtained by the JAWS program that has 2 DNAzymes, one in the 5 'end and another at the 3' end of the sequence (APTZ_AMP_J), and the same aptazyme obtained by JAWS but with one of the DNAzymes cut out from the sequence, located at 3 '(APTZ_AMP_JC). It was decided to cut the DNAzyme from this end to emulate the configuration of the aptazyme characterized in the literature.

The assays were performed in Flat-bottomed 96-well plates at different concentrations of triplicate AMP for each sequence and included a positive control; a triplicate of DNAzyme. The experimental scheme is presented in figure 1. Table I (notebook) shows the final concentration of each reagent in 100 μL and the volume in μL.

Here, the sequences worked in addition to the APTZ_AMP_P are presented:

APTZ_AMP_J

GGGTAGGGCGGGTTGGGgataaccttcCCTGGGGGAGTATTGCGGAGGAAGGTTatccccagcgGGGTAGGGCGGGTTGGG

APTZ_AMP_JC

GGGTAGGGCGGGTTGGGgataaccttcCCTGGGGGAGTATTGCGGAGGAAGGTTatccccagcg

See protocol in the notebook

Results of each tests are presented in figures 2, 3 and 4 for aptazymes “APTZ_AMP_P”, “APTZ_AMP_J” and “APTZ_AMP_JC” respectively, where the absorbance values have been plotted as function of time with duplicate for the first aptazyme and triplicated for the last two.

From these graphs we could conclude that the aptazyme “APTZ_AMP_JC” presents a dose dependence as does the “APTZ_AMP_P” aptazyme, while “APTZ_AMP_J” aptazyme did not have dose dependence. However the “APTZ_AMP_JC” aptazyme presented a greater range of error and / or variability than “APTZ_AMP_P” aptazyme.

First STX Aptazyme assay

Since the results of enzymatic assays with AMP aptazymes showed that the JAWS program generates sequences that can be efficient to detect ligands in a dose-dependent manner giving a colorimetric response when the sequences contain only one DNAzyme (APTZ_AMP_JC), they were sent to synthesize the following Aptazymes sequences:

APTZ_J1_LY

Aptazyme that better results showed last year:

GGGTAGGGCGGGTTGGGCATCGAGAAATTGAGGGTCGCATCCCGTGGAAACAGGTTCATTGGTGTTCGGCC

APTZ_STX_J1C

Aptazyme obtained through JAWS this year:

GGGTAGGGCGGGTTGGGCTCCGGTGGATTGAGGGTCGCATCCCGTGGAAACAGGTTCATTGGAGCCAAGGC

APTZ_STX_J2C

Aptazyme obtained through JAWS this year:

GGGTAGGGCGGGTTGGGGACTAAGGGATTGAGGGTCGCATCCCGTGGAAACAGGTTCATTGGGCCCTAGCC

Okadaic acid Aptazyme (the sequences of this last toxin were not tested so they will not be included in this record).

The tests were carried out with the 3 aptazymes of STX sent to be synthesized in a flat-bottomed 96-well plate.

See protocol in the notebook

Here are the results:

From these results, there was no evidence of a dependence dose by the aptazymes. It was also thought that the erratic behavior of some curves, as well as experimental error, may be due to the fact that the Aptazymes were active before starting the reaction, so it was proposed to perform the experiment with a variation in the protocol in the cooling stage.

3. AMP Aptazyme on filter papers

Lyophilization on filter papers

This experiment was carried out with the objective of evaluating whether ABTS oxidation reaction, which had already shown a dependence dose in the plaque assays, was capable of occurring when subjecting the aptazyme APTZ_AMP_P to the lyophilization process on Whatman N°1 filter paper. This filter paper was used given that it is known to generate an adequate environment for reactions involving DNA (like transcjription and translation of sequences) [4][5].

See protocol of Estimation of filter paper capacity and Lyophilized Preparation in the notebook.

Evaluation of DNAzymatic activity

See protocol in the notebook

Below are some images of the papers after 20 minutes. It would be expected that if the reaction were effective, the papers would show a detectable color gradient by direct observation.

In no case was an observable color detected in the lyophilized papers and subsequently re-hydrated, even when reviewing the papers the next day.

As a conclusion of previous result, it was thought to perform the same lyophilization operation but this time with each reagent 3 times more concentrated. In addition, in order to corroborate that the paper achieves dyeing, it was proposed to carry out an enzymatic assay on a plate and then smear papers in order to see if they achieve staining with the concentrations originally used.

Lyophilization at higher concentrations

See protocol in the notebook.

Below are some images of the papers during the course of 20 minutes. It would be expected that if the reaction were effective, the papers would show a detectable color gradient by direct observation.

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 <center><p style="width:70%"><b>From these results it was found that the concentration of reagents used is insufficient so that at the end of the reaction a staining of the papers with the given dimensions is generated.</b>
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 <center><p style="width:70%"><b>References:</b></p></center>
 <center><p style="width:70%">[1] Teller, C., Shimron, S., & Willner, I. (2009). Aptamer−DNAzyme hairpins for amplified biosensing. Analytical chemistry, 81(21), 9114-9119.</p></center>
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 <center><p style="width:70%">[5] Gomez, L. M., & Uribe, S. I. (2007). Preservation and storage of butterfly DNA using filter paper. Revista Colombiana de Entomología, 33(2), 191-196.
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