Team:Vilnius-Lithuania/Labjournal

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Parts construction

Part: P14.2 (BBa_K1773006)

Written by: IR
Performed by: ŠT, IR, MB, IS.

About

pLac+cI.
P10 and P11 plasmids are used. pLac (P11) and repressor cI (P10) ligation.

Date	Materials	Experiment
06 30	P10 P11	P10 and P11 transformation into DH5α.
07 01		Bacteria inoculation (4 minipreps).
07 09	P10 P11	Plasmids’ restriction (3 ug each). P10 with EcoRI and XBal (+FastAp). P11 with EcoRI and SpeI. Extraction from gel L10 and L11 are produced. Conc.: L11 – 2,4 ng/uL.

Conclusions and Results:

07 14 – all of the colonies are successful, except third colony.

Parts construction

Part: P15.1 (BBa_)

Written by: IR
Performed by: ŠT, IR, MB, IS.

About

Cas3 with mutated restriction sites
L7+L15. Concentration - 261 ng/μL

Date	Materials	Experiment
06 30	P13 P7	P13 and P7 transformation into DH5α.
07 01		Transformants are inoculated (4 minipreps each).
07 02		Plasmid extraction. Concentrations: P7 – 174,1 ng/μL and 166 ng/μL. P13 - 216 ng/μL and 131, 5 ng/μL.
07 13	P13	Cas3 mutagenesis (with ST1/2, ST3/4, ST5/6 primers).
07 16	Mutated P13	Cas3 plasmids extraction.
07 21-23	Mutated P13	Restriction with EcoRI, XbaI and PstI.
07 27	Mutated P13	Cas3 mutagenesis.
07 29	P7	Restriction with EcoRI and SpeI. L7 is produced.
07 31	P13
08 02	Mutated P13	Mutated Cas3 restriction with EcoRI, XbaI and PstI.
08 05	Mutated P13	Cas3 mutagenesis.
08 07	Mutated P13	Mutated Cas3 restriction with PstI. Mutagenesis was successful. L15 is produced.
08 11	L7 L15	L7 and L15 ligation with pSB1C3 (EcoRI+XBal+FastAp). P15.1 is produced.
	P15.1	Sequencing.

Conclusions and Results:

07 21 – Mutagenesis was unsuccessful.
08 02 – successfully mutagenized EcoRI and XbaI sites.
08 07 – successful mutagenesis confirmed (XbaI and EcoRI sites are mutated).
08 07 – Successful mutagenesis (PstI, XbaI and EcoRI sites are mutated).

Parts construction

Parts: P26, P27, P28, P29 (BBa_)

Written by: IR
Performed by: ŠT, IR, BB, IS.

About

P26 – L7+L26 pLux/cI+SRBS
P27 – L7+L27 pLux/cI+MRBS
P28 – L7+L28 pLux/cI+WRBS
P29 – L7+L29 pLux/cI

Date	Materials	Experiment
07 27	ST9 ST10 ST11 ST12 ST15 ST16 ST17 ST18 ST19 ST20	pLux/cI contruction from oligos – PCR reaction with ST9 and ST10/11/12 primers, then with ST15 and ST16/17/18. Parallel PCR with ST9 and ST19 and then with ST15 and ST20. PCR products purification.
07 28		PCR products from oligos restriction with EcoRI and SpeI. L26, L27, L28 and L29 are produced.
07 28	L7 L26 L27 L28 L29	Ligation of: L7 and L26, L7 and L27, L7 and L28, L7 and L29 and their transformation into DH5α.
07 29 - - 08 05		L7+L26 colony PCR with ST15 and VR. L7+L27 colony PCR with ST15 and VR. L7+L28 colony PCR with ST15 and VR. 1st and 2nd colonies are inoculated. P26, P27, 28 and P29 are produced P26, P27, 28 and P29 restriction with NspI.
08 10		P26, P27, 28 and P29 sequencing with VF2.

Conclusions and Results:

07 31 – all of the colonies are successful.
08 10 – all biobricks are sequenced succesfully.

Parts construction

Part: P30 (BBa_)

Written by: IR
Performed by: ŠT

About

cI repressor promoter (BBa_R1051) (P4) + screen plasmid intermediate (GFP gene) (BBa_I13504) (P5).

Date	Materials	Experiment
06 30	P14	P4 transformation into DH5α.
07 01		Bacteria inoculation (4 minipreps).
07 02	P4	Plasmid extraction. Concentrations: P4 - 238,3 ng/μL and 224,3 ng/μL. P4 restriction with EcoRI and XBal. Extraction from gel. L4 is produced (con. 16,2 ng/μL).
07 07	P5	P5 transformation into DH5α. Bacteria inoculation.
07 08		P5 plasmid extraction (P5.1, P5.2, P5.3, P5.4, P5.5 are produced).
07 29	P5.1 and P5.3	Restriction with EcoRI and SpeI. Extraction from gel. L5.1A, L5.1B, L5.1C and L5.3A, L5.3B, L5.3C are produced. Conc.: L5.1A – 0,6 ng/μL, L5.1B – 0,6 ng/μL, L5.1C – 2,4 ng/μL, L5.3A – 0,7 ng/μL, L5.3B - 3 ng/μL, L5.3C – 5,1 ng/μL. Ligation of L4 and L5.1, L4 and L5.3. P30 is produced.
08 01	P30	Sequencing.

Conclusions and Results:

07 09 – fragments were not the right ones.
07 29 – the right fragments are produced.

Parts construction

Part: P35, P36, P37 (BBa_)

Written by: IR
Performed by: ŠT, IR, BB, IS.

About

P35 - pLux/cI+SRBS(Strong RBS)+Cas3 (L26+L15.1)
P36 - pLux/cI+MRBS(Medium RBS)+Cas3 (L27+L15.1)
P37 - pLux/cI+WRBS(Weak RBS)+Cas3 (L28+L15.1)
P26 – L7+L26 (pLux/cI+SRBS)
P27 - pLux/cI+MRBS(Medium RBS)
P28 - pLux/cI+WRBS(Weak RBS)

Date	Materials	Experiment
07 28	P15	Mutated Cas3 with Preffix and Suffix restriction with EcoRI and XbaI. L15 is produced.
07 28	P26 P27 P28	PCR products from oligos restriction with EcoRI and SpeI. L26, L27, L28 and L29 are produced.
07 28	L15 L26 L27 L28	Ligation of: L15 and L26, L15 and L27, L15 and L28, and their transformation into DH5α.
07 29 - - 08 05		L7+L26 colony PCR with ST15 and VR. L7+L27 colony PCR with ST15 and VR L7+L28 colony PCR with ST15 and VR 1st and 2nd colonies are inoculated. P35, P36 and P37are produced P35, P36, P37 restriction with NspI.
08 10		P35, P36, P37 sequencing.

Conclusions and Results:

07 31 – all of the colonies are successful.
08 10 – all biobricks are sequenced succesfully.

Parts construction

Part: Cd1 (BBa_)

Written by: IR
Performed by: ŠT, IR, MB, IS, IO.

About

Mutated Cascade protein.

Date	Materials	Experiment
06 30	Cd	Cd transformation into DH5α.
07 01		Transformants are inoculated (4 minipreps each).
07 02		Plasmid extraction. Conc.: 329 ng/μL and 294 ng/μL.
07 14	Cd	Cd mutagenesis (with ST13/14 primers).
07 16 - 17		Mutated plasmids extraction. Restriction with EcoRI.
07 19	Mutated Cd	Restriction repeat.
07 21	Mutated Cd	Repeated mutagenesis (with ST13/14).
07 27	Mutated Cd	Mutated plasmids extraction. Mutated Cd restriction.
08 10	Mutated Cd L7	PCR with mutated Cd with ST26/27. PCR product purification. Conc.: 63 ng/μL. Restriction with EcoRI and SpeI. Mutated Cd ligation with L7. Cd1 is produced.
	Cd1	Sequencing.

Conclusions and Results:

07 16-17 – Mutagenesis was unsuccessful.
07 27 – Mutagenesis conformed as a successful.

Parts construction

Parts: 26-Cd, 27-Cd, 28-Cd (BBa_)

Written by: IR
Performed by: ŠT

About

26-Cd - Cascade with SRBS
27-Cd - Cascade with MRBS
28-Cd - Cascade with WRBS

Date	Materials	Experiment
08 15	Cd1	Mutated .......... with Preffix and Suffix restriction with EcoRI and XbaI. L35 is produced.
08 15	P26 P27 P28	PCR products from oligos restriction with EcoRI and SpeI. L26, L27, L28 and L29 are produced.
08 15	L35 L26 L27 L28	Ligation of: L35 and L26, L35 and L27, L35 and L28, and their transformation into DH5α.
08 17 - - 08 20		L35+L26 colony PCR with ST15 and VR. L35+L27 colony PCR with ST15 and VR L35+L28 colony PCR with ST15 and VR 1st and 2nd colonies are inoculated. 26-Cd, 27-Cd and 28-Cd are produced. 26-Cd, 27-Cd and 28-Cd restriction with NspI.
08 21		26-Cd, 27-Cd and 28-Cd sequencing.

Conclusions and Results:

07 31 – all of the colonies are successful.
08 10 – all biobricks are sequenced succesfully.