Difference between revisions of "Team:UCLA/Notebook/Honeybee Silk"

Revision as of 03:58, 15 May 2015

iGEM UCLA

Honeybee Silk Notebook

May 10 - May 16

May 11 Sequencing of silk biobricks

Today we sent in both our constructs to GeneWiz for sequencing.

For sequencing primers, I used the igem vf2 primers and vr primers that bind to the psb1c3 backbone, as well as a sequencing primer that we designed to bind to the silk sequence (p13) see https://benchling.com/s/p7bClpzQ/edit
The sequencing results came back and checked out for sample 1 of construct 1 (silk coding region) and samples 1 and 2 for construc 2 (regulatory elements + silk) i.e. we have our first honeybee biobricks!!!
For sequencing results of construct 1 see https://benchling.com/s/4XT6VRRU/edit (click on alignments on the right side of screen)
For sequencing results of construct 2 see https://benchling.com/s/TxD8z7Kq/edit (click on alignments on the right side of screen)

May 3 - May 9

April 26 - May 2

4/26 PCR off honey bee gene block

See Benchling for the g block sequence and primer reference code https://benchling.com/s/p7bClpzQ/edit
The goal of this is to clone 2 different constructs and prepare them as biobricks, one that is just the silk gene, and the other that as the promoter, rbs, etc.. required for protein expression.
Using primers p3, p7, and p8. (See Benchling link)

PCR Reaction 1 (q5 polymerase kit): primers honeybee p#7 and honeybee p#8 with gBlock, and honeybee p#3 and honeybee p#8 amplify just the honeybee coding region and the prom + coding region respectively

Component	Volume
5X Q5 Reaction Buffer	5
10 mM dNTPs	0.5
10 uM Forward (primer 3/7)	1.25
10 uM Reverse (primer 8)	1.25
Template (diluted to 1ng/uL)	0.5
Q5 High Fidelity DNA Polymerase	0.25
Nuclease Free Water	16.25

PCR program (using benchling annealing temperatures)

Temperature (C)	Time (Min:sec)
98	0:30
98 x 30 cycles	0:10
grad. 55.4/58.4/61.4 C x 30	0:20
72 x 30	0:30
72(diluted to 1ng/uL)	2:00
12	hold

The program and pcr reaction recipe were based on the manufacturer protocol. These annealing temperatures were determined using benchling's algorithm. In the future we will use the NEB annealing temperature calculator, because it is more accurate and takes the type of polymerase into account See tomorrow's entry for the gel image of the pcr reaction

4/27 visualization and purification of honeybee gblock PCR

We visualized the gradient pcr from 4/26 on a 1% agarose gel. See image below:

The PCR for both constructs (silk coding region) and (regulatory elements + silk coding region) worked relatively well across all gradient temperatures.
We next scaled up the PCR reaction to 50 ul for each construct and gel extracted the product
From left to right, just silk w/ bb prefix and suffix w/ increasing annealing temp. , ladder, followed by silk+ promoter at increasing temp (see 4/26 for pcr conditions)

4/28 PCR to prepare 2 honeybee constructs for cloning

We are repeating the same PCR from 4/26, but only at one temperature instead of a gradient, and we are scaling the reaction up to 50 ul.

PCR recipe

Component	Volume
5X Q5 Reaction Buffer	10
10 mM dNTPs	1.0
10 uM Forward (primer 3/7)	2.5
10 uM Reverse (primer 8)	2.5
Template (diluted to 1ng/uL)	1.0
Q5 High Fidelity DNA Polymerase	0.50
Nuclease Free Water	32.5

PCR program (using benchling annealing temperatures)

Temperature (C)	Time (Min:sec)
98	0:30
98 x 30 cycles	0:10
grad. 62 (silk) 58.4 (silk+prom) x 30	0:20
72 x 30	0:30
72(diluted to 1ng/uL)	2:00
10	hold

PCR products run on 1% agarose gel.

There were some non specific bands, but the appropriate bands were present. However, the bands were kind of off. I think this is due to the samples running weird on the gel. B/c the first two lanes were the exact same sample, just aliquoted, and they ran fairly differently.

Performed a gel extraction and purified using Qiagen min elute gel extraction kit

Results : 115 ng/ ul for silk tube #1, 86 ng/ul tube #2 (8.8 ul each tube) 136 ng/ul promoter + silk

4/30 Double digest of Honeybee PCR product and ligation into PSB1C3 plasmid backbone

Vinson and Olivia already prepared ecor1 and pst1 digested psb1c3, (35 ng/ul in honeybee box) which I will be using for ligation. It is column purified as well. I am double digesting both the plain silk construct, as well as the promoter+silk construct with ecoR1 and pst1.

Digestion Rxn (50 ul) One for silk and One for prom+silk

EcoR1 (C)	1 ul
Pst1	1 ul
NEB buffer 2.1 (10x)	5 ul
Silk DNA / PRom+Silk DNA	8.7 ul / 7.2 ul
H20	34.2 / 35.8 ul

@@ Line 237: / Line 237: @@
        </details>
+<details>
+         <summary> 4/30 Double digest of Honeybee PCR product and ligation into PSB1C3 plasmid backbone</summary>
+Vinson and Olivia already prepared ecor1 and pst1 digested psb1c3, (35 ng/ul in honeybee box) which I will be using for ligation. It is column purified as well.
+I am double digesting both the plain silk construct, as well as the promoter+silk construct with ecoR1 and pst1.
+<li>
+Digestion Rxn (50 ul)
+One for silk and One for prom+silk
+<table style="width: 100%">
+                  <tr>
+                     <td><b>EcoR1 (C)</b></td>
+                     <td>1 ul</td>
+                  </tr>
+                  <tr>
+                     <td><b>Pst1</b></td>
+                     <td>1 ul</td>
+                  </tr>
+                  <tr>
+                     <td><b>
+NEB buffer 2.1 (10x)
+</b></td>
+                     <td>5 ul</td>
+                  </tr>
+                  <tr>
+                     <td><b>
+Silk DNA / PRom+Silk DNA
+ </b>
+                     </td>
+                     <td>
+.7 ul / 7.2 ul
+</td>
+                  </tr>
+                  <tr>
+                     <td><b>
+                        H20
+                        </b>
+                     </td>
+                     <td>
+.2 / 35.8 ul
+</td>
+                  </tr>
+</table>
+</li>
+</details>
     </details>