Team:Bielefeld-Germany/Protocols

From 2011.igem.org

(Difference between revisions)

Latest revision as of 16:48, 15 September 2011

Molecular

Here you can read more about our methods for cloning and BioBrick assembly.

Genetic engineering is a basic tool of synthetic biology. With the help of standardized DNA building blocks it is comparatively easy to create new and modify existing natural systems. The methods we have used in our project to modify DNA are presented here

Production

These are the protocols for the cultivations and the downstream processing.

Before the work with a cell-free system based on biological material can start, the needed proteins for this have to be produced and purified first. These methods and the one's we used to characterize BioBricks ''in vivo'' are presented here

Analytics

Protocols for the analytical methods we used.

DNA and proteins are very small and cannot be seen by the naked eye. To control the success and the results of your upstream and downstream processes, analytical methods are necessary that give reliable results to make DNA or proteins in any way visible for you. The analytical methods we used in our project can be found here

Molecular Genetic engineering protocols
Production Upstreaming and downstreaming
Analytics Analytical methods

@@ Line 1: / Line 1: @@
 {{Bielefeld_2011_Header}}
-== Transformation via electroporation ==
+<html>
+<style type="text/css">
-* Thaw 50 µL competent ''E.coli'' cells on ice, dilute with icecold 50 µL glycerol (10 %) if necessary
+ul {
-* Add 0.5-5 µL plasmid to 50 µl electrocompetent cells
+    list-style-image:none;
-* Store cells on ice for 1 minute
+}
-* Electroporate at U = 2.5 kV, C = 25 µF, R = 200 Ώ
+#bodyContent{
-* Transfer transformation reaction to 450 µL SOC-Medium and shake 1 h at 37 °C
+    background-color: #D0D0D0;
-* Centrifuge 2 min at 800 rpm and plate on selective LB-Medium
+}
-==Transformation of Single Step (KRX) Competent Cells by Promega==
+</style>
-using [http://www.promega.com/~/media/Files/Resources/Protocols/Technical%20Bulletins/101/Single%20Step%20Competent%20Cells%20Protocol.ashx protocol for ''E. coli'' KRX single step competent cells by Promega]
-* Remove Single Step (KRX) Competent Cells from –70 °C, and place on ice for 5 minutes or until just thawed.
+<!-- tab panes -->
-* Add 1–50 ng of DNA (in a volume not greater than 5 μL) to the Single Step (KRX) Competent Cells. Move the pipette tip through the cells while dispensing. Quickly flick the tube several times. Do not vortex!
+<div id="panes">
-* Immediately return the tubes to ice for 5–30 minutes
-* Heat-shock cells for 15–20 seconds in a water bath at exactly 42 °C. Do not shake.
-* Immediately place the tubes on ice for 2 minutes.
-* Add 450 μL of room-temperature SOC medium to each transformation reaction, and incubate for 60 minutes at 37 °C with shaking (approximately 225 rpm). For best transformation efficiency, lay the tubes on their sides and tape them to the platform.
-* For each transformation reaction, we recommend plating 100 μL of undiluted cells and 1:10 and 1:100 cell dilutions on antibiotic plates. Incubate the plates at 37 °C overnight.
-== Standard BioBrick Assembly ==
+	<div>
+		<img src="https://static.igem.org/mediawiki/2011/thumb/1/1a/Bielefeld_Silver_1.png/300px-Bielefeld_Silver_1.png"  />
+		<h3>Molecular</h3>
-modified from [http://openwetware.org/wiki/Silver:_BB_Strategy Silver lab]:
+		<p class="more">
+			Here you can read more about our methods for cloning and BioBrick assembly.
+		</p>
+		<p>
+			Genetic engineering is a basic tool of synthetic biology. With the help of standardized DNA building blocks it is comparatively easy to create new and modify existing natural systems. The methods we have used in our project to modify DNA are presented <a href="https://2011.igem.org/Team:Bielefeld-Germany/Protocols/Genetics">here</a>
+		</p>
+	</div>
+	<div>
-This assembly method can be used for BioBricks which are bigger than 150 bp. The BioBrick should be at least 500 bp bigger or smaller than the backbone. The BioBrick, which complies with these conditions, is used as the insert and is assembled into the prefix or suffix of the other used BioBrick, called vector. So you have to differentiate between a prefix and a suffix insertion.
+		<img src="https://static.igem.org/mediawiki/2011/a/a1/Bielefeld-Germany2011-Fermenter-klein.jpg"  />
+		<h3>Production</h3>
+		<p class="more">
+			These are the protocols for the cultivations and the downstream processing.
+		</p>
+		<p>
+			Before the work with a cell-free system based on biological material can start, the needed proteins for this have to be produced and purified first. These methods and the one's we used to characterize BioBricks ''in vivo'' are presented <a href="https://2011.igem.org/Team:Bielefeld-Germany/Protocols/Downstream-processing">here</a>
+		</p>
+	</div>
-[[Image:Bielefeld_Silver_1.png|300px|thumb|right|Silver Suffix Insertion]]
+	<div>
-[[Image:Bielefeld_Silver_2.png|300px|thumb|right|Silver Prefix Insertion]]
-=== Suffix Insertion ===
+		<img src="https://static.igem.org/mediawiki/2011/a/a9/Bielefeld-Germany2011-MSwiki.jpg"  />
+		<h3>Analytics </h3>
+		<p class="more">
+			Protocols for the analytical methods we used.
+		</p>
+		<p>
+			DNA and proteins are very small and cannot be seen by the naked eye. To control the success and the results of your upstream and downstream processes, analytical methods are necessary that give reliable results to make DNA or proteins in any way visible for you. The analytical methods we used in our project can be found <a href="https://2011.igem.org/Team:Bielefeld-Germany/Protocols/Analytics">here</a>
+		</p>
+	</div>
-* Digestion of insert: at least 700 ng DNA / 10 µL volume, 1 µL 10x Tango buffer, 0.5 µL XbaI, 1 µL PstI. Digest for 2 h at 37 °C, afterwards inactivation for 20 min at 80 °C. Clean up the insert via gel electrophoresis. When cutting the insert out of the gel try to avoid staining or exposure to ultraviolet light of the insert.
+</div>
-* Digestion of vector about 700 ng DNA / 10 µL volume, 1 µL 10x orange buffer, 0.5 µL SpeI, 0.5 µL PstI. Digest for 2 h at 37 °C, afterwards inactivation for 20 min at 80 °C. Add 1 µL SAP (shrimp alcaline phosphatase) and 1.2 µL 10 x SAP buffer, incubate for 1 h at 37 °C. Clean up the vector with a PCR clean-up kit.
+<br clear="all" />
-* Ligation: after digestion and clean-up: 50 - 200 ng of vector, 3 - 10 fold molar access of insert, 20 µL ligation volume, 2 µL T4-Ligase-Buffer, 1 µL T4-Ligase. Incubate for 20 - 30 min at room temperature, afterwards inactivation for 5 min at 70 °C. Then: store at -20 °C or transform.
-=== Prefix Insertion ===
+<!-- navigator -->
+<div id="nav">
+	<ul style="list-style-type:none">
+		<li>
+			<a href="#1">
+				<img src="https://static.igem.org/mediawiki/2011/9/9a/Bielefeld-Germany2011-Thermocycler-klein.jpg"/>
+				<strong>Molecular</strong>
+				Genetic engineering protocols
+			</a>
+		</li>
+		<li>
+			<a href="#2">
+				<img src="https://static.igem.org/mediawiki/2011/2/27/Bielefeld-Germany2011-GFPtubes.jpg"/>
+				<strong>Production</strong>
+				Upstreaming and downstreaming
+			</a>
-* Digestion of insert: at least 700 ng DNA / 10 µL volume, 1 µL 10x BamHI buffer, 0.5 µL EcoRI, 0.5 µL SpeI. Digest for 2 h at 37 °C, afterwards inactivation for 20 min at 80 °C. Clean up the insert via gel electrophoresis. When cutting the insert out of the gel try to avoid staining or exposure to ultraviolet light of the insert.
+		</li>
+		<li>
+			<a href="#3">
+				<img src="https://static.igem.org/mediawiki/2011/6/6c/Bielefeld-Germany2011-analyticsklein.JPG" />
+				<strong>Analytics</strong>
+				Analytical methods
+			</a>
+		</li>
-* Digestion of vector about 700 ng DNA / 10 µL volume, 1 µL 10 x Tango buffer, 0.5 µL EcoRI, 0.5 µL XbaI. Digest for 2h at 37 °C, afterwards inactivation for 20 min at 80 °C. Add 1 µL SAP (shrimp alcaline phosphatase) and 1.2 µL 10 x SAP buffer, incubate for 1 h at 37 °C. Clean up the vector with a PCR clean-up kit.
+	</ul>
-* Ligation: after digestion and clean-up: 50 - 200 ng of vector, 3 - 10 fold molar access of insert, 20 µL ligation volume, 2 µL T4-Ligase-Buffer, 1 µL T4-Ligase. Incubate for 20 - 30 min at room temperature, afterwards inactivation for 5 min at 70 °C. Then: store at -20 °C or transform.
+</div>
-=== Variations ===
-* A digestion over night is possible. If you digest over night use only 0.1 µL restriction enzyme.
+<br clear="all" />
-* It is also possible to use PCR product as insert. Digest after PCR with corresponding restriction enzymes and clean up with PCR clean-up kit. This could lead to higher yields of insert DNA because a lot of DNA gets lost during the gel electrophoresis clean up.
+<script>
+$(function() {
-* Sometimes some BioBricks are hard to assemble. Then you have to clean up the vector by gel electrophoresis as well.
+	$("#nav ul").tabs("#panes > div", {effect: 'fade', fadeOutSpeed: 400});
-== Standard Freiburg BioBrick Assembly ==
+});
+</script>
-modified from [http://openwetware.org/wiki/Silver:_BB_Strategy Silver lab] and [http://partsregistry.org/Assembly_standard_25 Assembly standard 25]:
+</html>
-This assembly method can be used for fusion protein assemblies with BioBricks which are bigger than 150 bp. The BioBrick should be at least 500 bp bigger or smaller than the backbone. The BioBrick, which complies with these conditions, is used as the insert and is assembled into the prefix or suffix of the other used BioBrick, which is called vector and needs to be available in the BioBrick [http://partsregistry.org/Assembly_standard_25 Assembly standard 25]. You have to differentiate between a prefix and a suffix insertion.
-=== Suffix Insertion ===
-* Digestion of insert: at least 700 ng DNA / 10 µL volume, 1 µL 10x NEB buffer 4 + 0.1 µL 100x BSA, 0.5 µL NgoMIV (NEB), 1 µL PstI. Digest for 2 h at 37 °C, afterwards inactivation for 20 min at 80 °C. Clean up the insert via gel electrophoresis. When cutting the insert out of the gel try to avoid staining or exposure to ultraviolet light of the insert.
-* Digestion of vector about 700 ng DNA / 10 µL volume, 1 µL 10x orange buffer, 0.5 µL AgeI, 0.5 µL PstI. Digest for 2 h at 37 °C, afterwards inactivation for 20 min at 80 °C. Add 1 µL SAP (shrimp alcaline phosphatase) and 1.2 µL 10x SAP buffer, incubate for 1 h at 37 °C. Clean up the vector with a PCR clean-up kit.
-* Ligation: after digestion and clean-up: 50 - 200 ng of vector, 3 - 10 fold molar access of insert, 20 µL ligation volume, 2 µL T4-Ligase-Buffer, 1 µL T4-Ligase. Incubate for 20 - 30 min at room temperature, afterwards inactivation for 5 min at 70 °C. Then: store at -20 °C or transform.
-=== Prefix Insertion ===
-* Digestion of insert: at least 700 ng DNA / 10 µL volume, 1 µL 10x orange buffer, 0.5 µL EcoRI, 0.5 µL AgeI. Digest for 2 h at 37 °C, afterwards inactivation for 20 min at 80 °C. Clean up the insert via gel electrophoresis. When cutting the insert out of the gel try to avoid staining or exposure to ultraviolet light of the insert.
-* Digestion of vector about 700 ng DNA / 10 µL volume, 1 µL 10 x NEB buffer 4, 0.5 µL EcoRI, 0.5 µL NgoMIV (NEB). Digest for 2h at 37 °C, afterwards inactivation for 20 min at 80 °C. Add 1 µL SAP (shrimp alcaline phosphatase) and 1.2 µL 10 x SAP buffer, incubate for 1 h at 37 °C. Clean up the vector with a PCR clean-up kit.
-* Ligation: after digestion and clean-up: 50 - 200 ng of vector, 3 - 10 fold molar access of insert, 20 µL ligation volume, 2 µL T4-Ligase-Buffer, 1 µL T4-Ligase. Incubate for 20 - 30 min at room temperature, afterwards inactivation for 5 min at 70 °C. Then: store at -20 °C or transform.
-=== Variations ===
-* A digestion over night is possible. If you digest over night use only 0.1 µL restriction enzyme.
-* It is also possible to use PCR product as insert. Digest after PCR with corresponding restriction enzymes and clean up with PCR clean-up kit. This could lead to higher yields of insert DNA because a lot of DNA gets lost during the gel electrophoresis clean up.
-* Sometimes some BioBricks are hard to assemble. Then you have to clean up the vector by gel electrophoresis as well.
-==Standard 3A assembly==
-Modified from [http://ginkgobioworks.com/support/BioBrick_Assembly_Manual.pdf BioBrick Assembly Manual by Ginkgo BioWorks]
-===Digestion===
-* Thaw DNA from upstream and downstream part and the destination plasmid on ice.
-**  Destination plasmid has to carry the ''ccdB'' gene <partinfo>P1010</partinfo> as insert and has to have a different antibiotic resistance than the plasmids carrying the upstream and downstream parts
-**  DNA has to be cleaned (by MiniPrep or after a PCR)
-* 500 ng DNA / digestion mix for upstream part, downstream part and destination plasmid (total volume of mix 10 µL, dilute with ddH<sub>2</sub>0 if necessary)
-* Add 1 µL of 10x buffer and restriction enzymes as shown in the following table:
-<center>
-{|cellpadding="10" style="border-collapse: collapse; border-width: 1px; border-style: solid; border-color: #000"
-|-
-!style="border-style: solid; border-width: 1px"|
-!style="border-style: solid; border-width: 1px"| Upstream part
-!style="border-style: solid; border-width: 1px"| Downstream part
-!style="border-style: solid; border-width: 1px"| Destination plasmid
-|-
-|style="border-style: solid; border-width: 1px"| enzyme 1
-|style="border-style: solid; border-width: 1px"| 0.5 µL EcoRI
-|style="border-style: solid; border-width: 1px"| 0.5 µL XbaI
-|style="border-style: solid; border-width: 1px"| 0.5 µL EcoRI
-|-
-|style="border-style: solid; border-width: 1px"| enzyme 2
-|style="border-style: solid; border-width: 1px"| 0.5 µL SpeI
-|style="border-style: solid; border-width: 1px"| 1 µL PstI
-|style="border-style: solid; border-width: 1px"| 0.5 µL PstI
-|-
-|style="border-style: solid; border-width: 1px"| buffer
-|style="border-style: solid; border-width: 1px"| BamHI
-|style="border-style: solid; border-width: 1px"| Tango
-|style="border-style: solid; border-width: 1px"| Orange
-|}
-</center>
-* Incubation of the digestion mixes at 37 °C
-* After 2 h: add 0.5 µL SAP (shrimp alcaline phosphatase) and 1.15 µL 10x SAP buffer to destination plasmid mix, continue incubation at 37 °C
-* After another hour: heat inactivation of all mixes for 20 min at 80 °C
-* Continue with ligation or freeze the mixes
-===Ligation===
-* Ligation mix:
-** 2 µL ddH<sub>2</sub>O
-** 5 µL of every digestion mix (so 15 µL in total)
-** 2 µL T4-DNA-ligase buffer (thaw on ice!)
-** 1 µL T4-DNA-ligase
-* Incubate at least 20 min at room temperature, afterwards heat inactivation for 5 min at 70 °C (optional)
-* Freeze ligation mix or continue with transformation (heatshock or electroporation)
-==Freiburg 3A assembly==
-Modified from [http://ginkgobioworks.com/support/BioBrick_Assembly_Manual.pdf BioBrick Assembly Manual by Ginkgo BioWorks] and [http://partsregistry.org/Assembly_standard_25 Assembly standard 25]
-===Digestion===
-* Thaw DNA from upstream and downstream part (=N-terminal and C-terminal protein domain) and the destination plasmid on ice.
-**  Destination plasmid has to carry the ''ccdB'' gene <partinfo>P1010</partinfo> as insert and has to have a different antibiotic resistance than the plasmids carrying the upstream and downstream parts
-**  DNA has to be cleaned (by MiniPrep or after a PCR)
-* 500 ng DNA / digestion mix for upstream part, downstream part and destination plasmid (total volume of mix 10 µL, dilute with ddH<sub>2</sub>0 if necessary)
-* Add 1 µL of 10x buffer and restriction enzymes as shown in the following table:
-<center>
-{|cellpadding="10" style="border-collapse: collapse; border-width: 1px; border-style: solid; border-color: #000"
-|-
-!style="border-style: solid; border-width: 1px"|
-!style="border-style: solid; border-width: 1px"| Upstream part
-!style="border-style: solid; border-width: 1px"| Downstream part
-!style="border-style: solid; border-width: 1px"| Destination plasmid
-|-
-|style="border-style: solid; border-width: 1px"| enzyme 1
-|style="border-style: solid; border-width: 1px"| 0.5 µL EcoRI
-|style="border-style: solid; border-width: 1px"| 0.5 µL NgoMIV
-|style="border-style: solid; border-width: 1px"| 0.5 µL EcoRI
-|-
-|style="border-style: solid; border-width: 1px"| enzyme 2
-|style="border-style: solid; border-width: 1px"| 0.5 µL AgeI
-|style="border-style: solid; border-width: 1px"| 1 µL PstI
-|style="border-style: solid; border-width: 1px"| 0.5 µL PstI
-|-
-|style="border-style: solid; border-width: 1px"| buffer
-|style="border-style: solid; border-width: 1px"| Orange
-|style="border-style: solid; border-width: 1px"| NEB buffer 4 + BSA
-|style="border-style: solid; border-width: 1px"| Orange
-|}
-</center>
-* Incubation of the digestion mixes at 37 °C
-* After 2 h: add 0.5 µL SAP (shrimp alcaline phosphatase) and 1.15 µL 10x SAP buffer to destination plasmid mix, continue incubation at 37 °C
-* After another hour: heat inactivation of all mixes for 20 min at 80 °C
-* Continue with ligation or freeze the mixes
-===Ligation===
-* Ligation mix:
-** 2 µL ddH<sub>2</sub>O
-** 5 µL of every digestion mix (so 15 µL in total)
-** 2 µL T4-DNA-ligase buffer (thaw on ice!)
-** 1 µL T4-DNA-ligase
-* Incubate at least 20 min at room temperature, afterwards heat inactivation for 5 min at 70 °C (optional)
-* Freeze ligation mix or continue with transformation (heatshock or electroporation)
-== Restriction analysis ==
-* Digest BioBrick of interest: about 400 ng DNA / 10 µL volume, 1 µL 10x orange buffer, 0.5 µL NotI or PstI. Digest for 2 h at 37 °C. NotI is used to determine the length of the BioBrick and the plasmid backbone, PstI ist used to determine the length of the BioBrick in the plasmid backbone.
-* Gel electrophoresis: add 2 µL loading buffer to every digestion mix, apply about 100 - 200 ng DNA / pocket in gel. Don't forget to apply the uncut BioBrick as well. A good agarose concentration for BioBricks between 0.2 and 3 kb is 1.5 %. The smaller your BioBrick of interest is the higher the agarose concentration should be and vice versa. The gel electrophoresis is made with TAE-buffer. Be sure that you melt your agarose gel in the same buffer you use for the electrophoresis later.
-== Colony PCR ==
-* Pick one colony with a sterile tip and elute it in 100 µL ddH<sub>2</sub>0 or medium
-* Store the colony in 4 °C while colony PCR is running
-* One reaction mix contains:
-** 10 µL 5x buffer
-** 2 µL MgCl<sub>2</sub> (25 mM stock)
-** 1 µL dNTPs
-** 0.5 µL primer mix (prefix/suffix primers or sequencing primers)
-** 35.25 µL ddH<sub>2</sub>O
-** 0.25 µL GoTaq polymerase (Promega)
-** 1 µL template
-* PCR program:
-** Start: 3 min, 98 °C
-** 30 cycles of:
-*** 30 s, 98 °C
-*** 30 s, 55 °C
-*** 30 s / 1 kb template, 72 °C
-** Finish: 5 min, 72 °C
-* Gel electrophoresis: check the fragment size
-* Plate the correct colony
-==Bisphenol A analysis==
-===Extraction with ethylacetate===
-* mix 100 µL culture supernatant with 100 µL internal standard (bisphenol F, 100 µg L<sup>-1</sup>)
-* add 200 µL ethylacetate (HPLC grade) for extraction
-* vortex (30 s)
-* centrifuge for phase separation (5 min, 5000 g)
-* take a bit from upper phase and put it in a clean eppi
-* SpeedVac at 40 °C to remove ethlyacetate
-* solve remaining BPA in water (HPLC grade), vortex (30 s)
-* solubility of BPA in water only 300 mg L<sup>-1</sup>
-** for LC-MS analysis of BPA, 300 mg BPA L<sup>-1</sup> is definitely enough
-** if you want to detect or expect higher concentrations of BPA, solve it in an acetonitrile-water-mix
-===HPLC method===
-* C18 reverse phase column
-* gradient starting with 45 % acetonitrile up to 95 % acetonitrile
-==NAD<sup>+</sup> detection==
-For the [http://www.molecular-beacons.com/MB_SC_design.html design of Molecular Beacons] different available tools may help you so that a correct functionality is ensured under defined assay conditions. All measurements were made in the [https://2011.igem.org/Team:Bielefeld-Germany/Protocols#NAD.2B_bioassay_buffer NAD<sup>+</sup> bioassay buffer].
-===Characterisation of Molecular Beacons===
-Preferentially, use a complementary oligonucleotide (target) as well as two enshortened oligonucleotides (split target) for [http://www.molecular-beacons.com/MB_SC_protocol.html#cap3 characterising the Molecular Beacon] in its closed and open state. In this way you can verify simultaneously the ineffectiveness of the split target to reach the Molecular Beacon`s open state.
-* Optimal wavelengths:
-** Determine the emission spectrum of your Molecular Beacon by initially using a literature value for the exctintion wavelength of the labeled fluorophore. For this add 10 µL of 1 µM Molecular Beacon in 200 µL [https://2011.igem.org/Team:Bielefeld-Germany/Protocols#NAD.2B_bioassay_buffer NAD<sup>+</sup> bioassay buffer], mix thoroughly and wait 2 min until measuring the fluorescence with a spectrofluorometer at an defined temperature (optimally 37 °C) .
-** Add 10 µL of 2 µM either target or split target and shake at least 6 min until measuring the fluorescence again (when equilibrium is reached).
-** Repeat the procedure to determine the extinction spectrum using the self-calculated optimal emission wavelength for your fluorophore/quencher combination. For further fluorescence measurements use the extinction wavelength for which the difference between the Molecular Beacons's closed state and the open state signals is maximal.
-* Thermal profile analysis:
-** Prepare a 30 µL reaction mix composed of [https://2011.igem.org/Team:Bielefeld-Germany./Protocols#NAD.2B_bioassay_buffer NAD<sup>+</sup> bioassay buffer] and 1 µM Molecular Beacon. In a separate sample add 2 µM either target or split target.
-** Use a spectrofluorometric thermal cylcer to dertemine the fluorescence as a function of temperature. Start at 80 °C and decrease the temperature stepwise in 1 °C intervals holding each temperature for 1 min and measuring the fluorescence at the end of each step.
-* Signal-to-background ratio (S/B):
-[[Image:Bielefeld-Germany-2011 MB S-B-ratio.png|200px|thumb|right|Signal-to-background ratio]]
-**The approach is quite similar to the one that determines the optimal wavelengths which should be used to monitor the fluorescence of the [https://2011.igem.org/Team:Bielefeld-Germany/Protocols#NAD.2B_bioassay_buffer NAD<sup>+</sup> bioassay buffer] (F<sub>buffer</sub>) and the added Molecular Beacon (F<sub>closed</sub>) as well as the target (F<sub>open</sub>) or split target. Monitor the fluorescence until the equilibrium is reached each time before you add a new component.
-** The signal-to-background ratio can be calculated as shown on the right. Finally, compare the signal-to-background ratios after adding the target and split target to check whether the split target has an effect on the melting of the Molecular Beacon's hairpin structure.
-* Imaging:
-** Prepare a 200 µL reaction mix composed of [https://2011.igem.org/Team:Bielefeld-Germany./Protocols#NAD.2B_bioassay_buffer NAD<sup>+</sup> bioassay buffer] and 500 nM Molecular Beacon in a PCR tube. In a separate sample add 600 µM either target or split target. Excitate the samples by a UV transilluminator and take images preferably with a camera that can detect different colours.
-===Purification of DNA Ligase===
-===NAD<sup>+</sup> bioassay===
-==Used enzymes==
-{| class="wikitable" style="text-align:left"
-|-
-! Enzyme !!  style="padding-left:5px;" |Producer
-|-
-| GoTaq DNA-polymerase ||  style="padding-left:5px;" |Promega
-|-
-| KOD Hotstart DNA-polymerase ||  style="padding-left:5px;" |Novagen
-|-
-| NgoMIV ||  style="padding-left:5px;" |NEB
-|-
-| OneTaq DNA-polymerase ||  style="padding-left:5px;" |NEB
-|-
-| Pfu DNA-polymerase ||  style="padding-left:5px;" |Promega
-|-
-| Phusion HF DNA-polymerase ||  style="padding-left:5px;" |Finnzymes
-|-
-| Restriction enzymes (except NgoMIV)   ||  style="padding-left:5px;" |Fermentas
-|-
-| Shrimp alcaline phosphatase ||  style="padding-left:5px;" |Fermentas
-|-
-| T4-DNA-Ligase ||  style="padding-left:5px;" |Fermentas
-|-
-| ''taq'' DNA-polymerase ||  style="padding-left:5px;" |Bioline
-|-
-|}
-==Used Kits==
-{| class="wikitable" style="text-align:left"
-|-
-! Function !! style="padding-left:5px;" | Name
-|-
-| Plasmid purification || style="padding-left:5px;" | Fermentas GeneJET™ Plasmid Miniprep Kit
-|-
-| Plasmid purification || style="padding-left:5px;" | Promega PureYield™ Plasmid Preps
-|-
-| PCR Cleanup || style="padding-left:5px;" | Macherey Nagel NucleoSpin® Extract II
-|-
-| PCR Cleanup || style="padding-left:5px;" | Promega Wizard® SV Gel and PCR Clean-Up
-|-
-|}
-==Media, buffer, solutions etc.==
-===TAE buffer===
-For 1 L of 50 x TAE buffer you need:
-* 242.48 g Tris
-* 41.02 g Sodiumacetate
-* 18.612 g EDTA
-* Adjust pH to 7.8 with acetic acid
-* Solve in dH<sub>2</sub>O
-mL of the stock is diluted in 1 L dH<sub>2</sub>O for the gel electrophoresis (0.5 x TAE buffer).
-===DNA loading buffer===
-* 50 % (v/v) glycerol
-* 1 mM EDTA
-* 0.1 % (w/v) bromphenol blue
-* Solve in ddH<sub>2</sub>O
-===LB medium===
-For 1 L of LB medium you need:
-* 10 g Trypton
-* 5 g yeast extract
-* 10 g NaCl
-* 12 g Agar-Agar (for plates)
-* Adjust pH to 7.4
-===NAD<sup>+</sup> bioassay buffer===
-* 50 mM Tris-HCl, pH 8.0
-* 10 mM MgCl<sub>2</sub>
-* 2,5 mM CaCl<sub>2</sub>
-* 5 mM DTT
-* 0,05 % BSA
-==Used chemicals==
-{| class="wikitable" style="text-align:left"
-|-
-! Chemical !! style="padding-left:5px;" | Producer !! style="padding-left:5px;" | Purity
-|-
-| Acetonitrile || style="padding-left:5px;" | [https://de.vwr.com/app/catalog/Product?article_number=20048.320 VWR] || style="padding-left:5px;" | 99.9 %, HPLC Grade
-|-
-| Bisphenol F || style="padding-left:5px;" | [http://www.alfa.com/de/GP100W.pgm?DSSTK=A11417&rnd=097380668 Alfa Aesar] || style="padding-left:5px;" | 98 %
-|-
-| Ethylacetate || style="padding-left:5px;" | [https://de.vwr.com/app/catalog/Product?article_number=23882.321 VWR] || style="padding-left:5px;" | > 99.5 %, ''p.a.''
-|-
-| Chemical A || style="padding-left:5px;" | [http://www.link.com Producer A] || style="padding-left:5px;" | XX.X %
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