Difference between revisions of "Part:BBa K5492712"
('Fishing Method' With Aptamers)
 
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===<span class='h3bb'>Sequence and Features</span>===
+
===Experiments===
  
https://static.igem.wiki/teams/5492/registry/aptamer-beads-illustr-small.jpg
+
 
 +
==Transdermal device==
 +
The transdermal device and its usage are written in our protocol in the Experiment topic under
 +
the title “Transdermal transport of the enzymes and aptamers”. Please refer that [https://2024.igem.wiki/termosz-selye-hun/experiments paper] for details. Here we emphasize only the final measurement which is a truly simple A260 measurement.
 +
We received back from our team members three series of 300 uL volume samples which
 +
contained the aptamers packaged in liposomes and dispersed in the hydrogel. We also received
 +
two series dispersed in hydrogel without packaging them in liposomes. Each sample series
 +
consists of six 300 uL samples arriving to the acceptor phase after 1, 2, 4, 8, 12 and 24 hours.
 +
 
 +
Before the transdermal experiment we dissolved altogether 552.7 ug DNA aptamers dissolved in
 +
1200 uL TE buffer. From this amount 200 uL was used and was evenly distributed among the
 +
five, one-day-long (24 h) transdermal experiment. This means that in each of the five experiments
 +
we used 1/5*(200/1200)*552.7 = 18.42 ug aptamers at the donor phase.
 +
We determined the DNA content of the acceptor phase by measuring A260 values with
 +
Thermofisher Nanodrop device. The results were the following:
 +
 
 +
https://static.igem.wiki/teams/5492/registry/aptamers/allapt-1.png
 +
https://static.igem.wiki/teams/5492/registry/aptamers/allapt2.png
 +
 
 +
 
 +
 
 +
The following graph shows the 5 data series results:
 +
 
 +
https://static.igem.wiki/teams/5492/registry/aptamers/allapt-3.png
 +
 
 +
As it is clearly visible there are no precise trends in these results. Though the second experiment
 +
shows a large peak after eight hours, the other two control experiments don’t represent the same,
 +
so we can conclude that there is no evidence for a trend-like transdermal transport amongst
 +
aptamers in these experiments. It is still worth it to consider the summed-up transmission:
 +
 
 +
https://static.igem.wiki/teams/5492/registry/aptamers/allapt-4.png
 +
 
 +
Considering the exact, total amount of the transmission, we can recognize that only 3-6 ‰ of the
 +
aptamers went through the ex vivo membrane, which means that this method is not proper
 +
topical use of the aptamers.
 +
 
 +
 
 +
=='Fishing Method' With Aptamers==
 +
 
 +
Our original idea was to create a sustainable tool for usage other than the topical methods. For
 +
example, foods / alimentary liquids may contain histamine, causing inflammatory bowel disease
 +
or symptoms. If we could prove that the chosen aptamers can bind to the histamine molecules,
 +
we would be able to avoid using DAO or HNMT enzymes, which may be harmful for many
 +
reasons. However, using aptamers to cage histamine would mean the food will contain this extra
 +
amount of DNA. Usually, it is not dangerous, but removing the aptamers from the food after
 +
they fulfil their role would be better. We found out that in these cases aptamers should be
 +
elongated with a short extra sequence.
 +
The method’s essence is that the (strept)avidin on the surface of the beads can bind biotylinated
 +
ssDNA, the sequence of which are reversely complement with the elongated part of the aptamer.
 +
When we apply strong magnetic field, we expect to gather not only the beads, but together with
 +
them the elongated aptamers, too. These aptamers can trap the histamine, bind to the magnetic
 +
beads’ connector sequence and thus the histamine itself can be purified from the liquid. This
 +
scenario is depicted on the following figure:
 +
 
 +
https://static.igem.wiki/teams/5492/registry/aptamers/fishing/beads-1.png
 +
 
 +
As our budget could not cover the enough sensitive histamine assay to test our idea, we decided
 +
to do it in two parts. Firstly, we proved that these beads can attach the elongated aptamers and
 +
secondly we proved that the elongated aptamers can bind the histamine successfully.
 +
 
 +
Bead binding experiment:
 +
 
 +
We started with fully saturating the beads’ avidin’ spaces with the biotylinated connectors in two
 +
steps. We tracked the process by A260 measurement. The experimental results are here:
 +
 
 +
https://static.igem.wiki/teams/5492/registry/aptamers/fishing/beads-2.png
 +
 
 +
https://static.igem.wiki/teams/5492/registry/aptamers/fishing/beads-3.png
 +
 
 +
Then, we used 200 uL beads (1.2 mg beads in each reaction) to 50 uL elongated aptamers. The
 +
results were the following:
 +
 
 +
https://static.igem.wiki/teams/5492/registry/aptamers/fishing/bead-4.png
 +
 
 +
This means that the average binding capacity of the ssDNA coated beads is
 +
cca. 500 ng DNA / 1mg connector-coated beads.
 +
 
 +
The second part was to prove that the elongated aptamers are capable to trap the histamine
 +
molecules. To check this hypothesis, we used three different dilutions of histamine: 1 uM; 10 uM;
 +
100 uM. We added 50 uL of these solutions to 200 uL elongated aptamer solutions of which the
 +
concentration was 600 ng/uL. During the experiment we followed the procedure described in the
 +
Yokobayashi paper with two important modifications:
 +
After checking the folding of our aptamers via Mfold we recognised that the aptamers are
 +
more stable in solutions with high Mg2+ concentration. Therefore we used Thermofisher
 +
Dreamtaq Buffer with high MgCl2 concentration instead of the buffer proposed by the
 +
paper.
 +
 
 +
We used 65°C as unfolding temperature instead of the paper’s 55°C. The reason for this is
 +
that we learned from Mfold that the elongated aptamers have higher Tm in themselves.
 +
Finally, the cooled down solutions were used in the MAK432 colorimetric Histamine Assay Kit
 +
(from Sigma Aldrich).
 +
The allocation of the plate wells was the following (A1-A2 to H1-H2 were the standards; H10;
 +
H100 and H1000 represents reference with 10; 1000 and 1000 uM histamine solutions.
 +
Y=Yokobayashi a9 aptamer; J=Johnson’s H1 aptamer; S= Sullivan’s H5 aptamer – all in
 +
elongated form (see the [https://2024.igem.wiki/termosz-selye-hun/all-parts registry] for sequence details.)
 +
 
 +
https://static.igem.wiki/teams/5492/registry/aptamers/fishing/beads-5.png
 +
 
 +
https://static.igem.wiki/teams/5492/registry/aptamers/fishing/bead-6.png
 +
 
 +
And the numerical results:
 +
 
 +
https://static.igem.wiki/teams/5492/registry/aptamers/fishing/beads-7.png
 +
 
 +
Based on the above results it is obvious that in the 100 uM histamine solution the aptamer could
 +
trap the cca. 80% histamine in all three types of the aptamers. This means, that the protocol is
 +
useful and based on the used concentration we can estimate that 120 ug can trap 5 nmol
 +
histamine successfully.
 +
Thus, we could prove in two steps that our “fishing” procedure is a viable idea to use in the
 +
future to remove histamine from alimentary fluids.
  
 
<partinfo>BBa_K5492712 SequenceAndFeatures</partinfo>
 
<partinfo>BBa_K5492712 SequenceAndFeatures</partinfo>

Latest revision as of 12:13, 2 October 2024


S1_aptamer

S1 ssDNA aptamer sequence designed to specifically bind to histamine. The overhang of the 5' end of the sequence is complementary to s1_aptamer_connector. The connector sequence contains a 5' biotin tag (5'biosg) that lets the sequence bind to an avidin-coated magnetic bead via avidin-biotin connection.

Usage and Biology

Aptamers are generally artificial ssDNA, RNA, or peptide oligomers which bind to specific target molecules. All ssDNA aptamers we utilise are proven to be able to bind specifically to histamine, thus preventing the binding of the molecule to a histamine receptor.

Experiments

Transdermal device

The transdermal device and its usage are written in our protocol in the Experiment topic under the title “Transdermal transport of the enzymes and aptamers”. Please refer that paper for details. Here we emphasize only the final measurement which is a truly simple A260 measurement. We received back from our team members three series of 300 uL volume samples which contained the aptamers packaged in liposomes and dispersed in the hydrogel. We also received two series dispersed in hydrogel without packaging them in liposomes. Each sample series consists of six 300 uL samples arriving to the acceptor phase after 1, 2, 4, 8, 12 and 24 hours.

Before the transdermal experiment we dissolved altogether 552.7 ug DNA aptamers dissolved in 1200 uL TE buffer. From this amount 200 uL was used and was evenly distributed among the five, one-day-long (24 h) transdermal experiment. This means that in each of the five experiments we used 1/5*(200/1200)*552.7 = 18.42 ug aptamers at the donor phase. We determined the DNA content of the acceptor phase by measuring A260 values with Thermofisher Nanodrop device. The results were the following:

allapt-1.png allapt2.png


The following graph shows the 5 data series results:

allapt-3.png

As it is clearly visible there are no precise trends in these results. Though the second experiment shows a large peak after eight hours, the other two control experiments don’t represent the same, so we can conclude that there is no evidence for a trend-like transdermal transport amongst aptamers in these experiments. It is still worth it to consider the summed-up transmission:

allapt-4.png

Considering the exact, total amount of the transmission, we can recognize that only 3-6 ‰ of the aptamers went through the ex vivo membrane, which means that this method is not proper topical use of the aptamers.


'Fishing Method' With Aptamers

Our original idea was to create a sustainable tool for usage other than the topical methods. For example, foods / alimentary liquids may contain histamine, causing inflammatory bowel disease or symptoms. If we could prove that the chosen aptamers can bind to the histamine molecules, we would be able to avoid using DAO or HNMT enzymes, which may be harmful for many reasons. However, using aptamers to cage histamine would mean the food will contain this extra amount of DNA. Usually, it is not dangerous, but removing the aptamers from the food after they fulfil their role would be better. We found out that in these cases aptamers should be elongated with a short extra sequence. The method’s essence is that the (strept)avidin on the surface of the beads can bind biotylinated ssDNA, the sequence of which are reversely complement with the elongated part of the aptamer. When we apply strong magnetic field, we expect to gather not only the beads, but together with them the elongated aptamers, too. These aptamers can trap the histamine, bind to the magnetic beads’ connector sequence and thus the histamine itself can be purified from the liquid. This scenario is depicted on the following figure:

beads-1.png

As our budget could not cover the enough sensitive histamine assay to test our idea, we decided to do it in two parts. Firstly, we proved that these beads can attach the elongated aptamers and secondly we proved that the elongated aptamers can bind the histamine successfully.

Bead binding experiment:

We started with fully saturating the beads’ avidin’ spaces with the biotylinated connectors in two steps. We tracked the process by A260 measurement. The experimental results are here:

beads-2.png

beads-3.png

Then, we used 200 uL beads (1.2 mg beads in each reaction) to 50 uL elongated aptamers. The results were the following:

bead-4.png

This means that the average binding capacity of the ssDNA coated beads is cca. 500 ng DNA / 1mg connector-coated beads.

The second part was to prove that the elongated aptamers are capable to trap the histamine molecules. To check this hypothesis, we used three different dilutions of histamine: 1 uM; 10 uM; 100 uM. We added 50 uL of these solutions to 200 uL elongated aptamer solutions of which the concentration was 600 ng/uL. During the experiment we followed the procedure described in the Yokobayashi paper with two important modifications: After checking the folding of our aptamers via Mfold we recognised that the aptamers are more stable in solutions with high Mg2+ concentration. Therefore we used Thermofisher Dreamtaq Buffer with high MgCl2 concentration instead of the buffer proposed by the paper.

We used 65°C as unfolding temperature instead of the paper’s 55°C. The reason for this is that we learned from Mfold that the elongated aptamers have higher Tm in themselves. Finally, the cooled down solutions were used in the MAK432 colorimetric Histamine Assay Kit (from Sigma Aldrich). The allocation of the plate wells was the following (A1-A2 to H1-H2 were the standards; H10; H100 and H1000 represents reference with 10; 1000 and 1000 uM histamine solutions. Y=Yokobayashi a9 aptamer; J=Johnson’s H1 aptamer; S= Sullivan’s H5 aptamer – all in elongated form (see the registry for sequence details.)

beads-5.png

bead-6.png

And the numerical results:

beads-7.png

Based on the above results it is obvious that in the 100 uM histamine solution the aptamer could trap the cca. 80% histamine in all three types of the aptamers. This means, that the protocol is useful and based on the used concentration we can estimate that 120 ug can trap 5 nmol histamine successfully. Thus, we could prove in two steps that our “fishing” procedure is a viable idea to use in the future to remove histamine from alimentary fluids.


Assembly Compatibility:
  • 10
    COMPATIBLE WITH RFC[10]
  • 12
    COMPATIBLE WITH RFC[12]
  • 21
    COMPATIBLE WITH RFC[21]
  • 23
    COMPATIBLE WITH RFC[23]
  • 25
    COMPATIBLE WITH RFC[25]
  • 1000
    COMPATIBLE WITH RFC[1000]