Team:NEFU China/Labnote

From 2014.igem.org

(Difference between revisions)
Line 136: Line 136:
           </table>
           </table>
           <p class="text-center"><strong>BCP or BRP(smtB, smtO-P and amilCP/RFP )</strong></p>
           <p class="text-center"><strong>BCP or BRP(smtB, smtO-P and amilCP/RFP )</strong></p>
-
           <p>The smt locus was successfully cloned from <em>Synechococcus elongates</em> PCC7942. <a href="#">Show sequence</a></p>
+
           <p>The smt locus was successfully cloned from <em>Synechococcus elongates</em> PCC7942. <a href="https://static.igem.org/mediawiki/2014/b/bc/Sequence_of_smt_locus.pdf">Show sequence</a></p>
           <p class="text-center"><img src="https://static.igem.org/mediawiki/2014/8/82/NEFU_CHINA_foundation_fig1.png" class="img-thumbnail"></p>
           <p class="text-center"><img src="https://static.igem.org/mediawiki/2014/8/82/NEFU_CHINA_foundation_fig1.png" class="img-thumbnail"></p>
           <p class="text-center">Fig.1 PCR product of the smt locus(640bp); Marker (DL2000)</p>
           <p class="text-center">Fig.1 PCR product of the smt locus(640bp); Marker (DL2000)</p>
Line 510: Line 510:
         <p>Gel Extraction with TIANgel Midi Purification Kit(TIANGEN BIOTECH)
         <p>Gel Extraction with TIANgel Midi Purification Kit(TIANGEN BIOTECH)
Ligation and transformation with pEASY-T5 Zero Cloning Kit from TransGen Biotech. The sequencing result is consistent with our designation.</p>
Ligation and transformation with pEASY-T5 Zero Cloning Kit from TransGen Biotech. The sequencing result is consistent with our designation.</p>
-
     <p>FC(Flocculation gene, CP25 and CDS7)<a href="#">show sequence</a></p>
+
     <p>FC(Flocculation gene, CP25 and CDS7)<a href="https://static.igem.org/mediawiki/2014/8/84/Sequence_of_Flocculation_gene%2C_CP25_and_CDS7.pdf">show sequence</a></p>
         <p>The flocculation gene was successfully cloned from <em>Bacillussp.  F2.</em></p>
         <p>The flocculation gene was successfully cloned from <em>Bacillussp.  F2.</em></p>
         <p>While CP25 and CDS7 and the backbone sequence adjacent to them was synthesized by BGI Tech.And they are inserted in pMV.</p>
         <p>While CP25 and CDS7 and the backbone sequence adjacent to them was synthesized by BGI Tech.And they are inserted in pMV.</p>
Line 856: Line 856:
           </tr>
           </tr>
         </table>
         </table>
-
<p>Transformation <a href="#">see protocol</a></p>
+
<p>Transformation <a href="https://static.igem.org/mediawiki/2014/f/f5/NEFU_China_Transformation.pdf">see protocol</a></p>
         <p>Colony PCR</p>
         <p>Colony PCR</p>
         <table align="center" class="MsoNormalTable" border="1" cellspacing="0" cellpadding="0" style="background:#F9F9F9;border-collapse:collapse;border:none;">
         <table align="center" class="MsoNormalTable" border="1" cellspacing="0" cellpadding="0" style="background:#F9F9F9;border-collapse:collapse;border:none;">
Line 2,470: Line 2,470:
<p class="text-center"><img src="https://static.igem.org/mediawiki/2014/e/e0/NEFU_China_project_fig15.png" class="img-thumbnail"></p>
<p class="text-center"><img src="https://static.igem.org/mediawiki/2014/e/e0/NEFU_China_project_fig15.png" class="img-thumbnail"></p>
<p><strong>Protein characterization</strong></p>
<p><strong>Protein characterization</strong></p>
-
<p>Protein characterization by SDS-PAGE. <a href="#">see protocol</a></p>
+
<p>Protein characterization by SDS-PAGE. <a href="https://static.igem.org/mediawiki/2014/d/d1/SDS-PAGE.pdf">see protocol</a></p>
<p class="text-center"><img src="https://static.igem.org/mediawiki/2014/d/de/NEFU_China_labnote_fig36.png" class="img-thumbnail"></p>
<p class="text-center"><img src="https://static.igem.org/mediawiki/2014/d/de/NEFU_China_labnote_fig36.png" class="img-thumbnail"></p>
<p>Fig.26 result of SDS-PAGE 1,2,3. Analysis of amilCP; 5,6,7. Annalysis of  RFP; 1&5. not induced; 2&6. Proteins from IPTG induced(0.8mM) <em>E.coli</em>.;  3&7. Control without reporter gene; 4. Protein marker</p>
<p>Fig.26 result of SDS-PAGE 1,2,3. Analysis of amilCP; 5,6,7. Annalysis of  RFP; 1&5. not induced; 2&6. Proteins from IPTG induced(0.8mM) <em>E.coli</em>.;  3&7. Control without reporter gene; 4. Protein marker</p>

Revision as of 07:35, 17 October 2014

Lab note

Abbreviations

B

smtB

Trans-acting regulator

OP

smtO-P

Smt operator/promoter region, a bi-directional promoter

A

smtA

Encoding MT-like protein that can sequester metal ions

C

amilCP

Encoding a chromoprotein that has a blue/purple color visible to the naked eye. A registered part from iGEM11_Uppsala-Sweden

R

RFP

Red Fluorescent Protein.
A registered part from iGEM11_Uppsala-Sweden

Flo

Flocculation gene

It can improve the flocculent activity of our host cells (Rosetta pLysS)

CP25

A constitutive strong promoter

CDS7

Encoding a short peptide that can bind to CdS and
induce the formation of CdS nanocrystals

BCP

According to priority: smtB, smtO-P(omit here), amilCP

BRP

According to priority: smtB, smtO-P(omit here), RFP

OPA

According to priority: smtO-P, smtA

FCDS7

According to priority: flocculation gene, CP25(omit here), CDS7

BCP or BRP(smtB, smtO-P and amilCP/RFP )

The smt locus was successfully cloned from Synechococcus elongates PCC7942. Show sequence

Fig.1 PCR product of the smt locus(640bp); Marker (DL2000)

BCP/BRP

Molecular biology techniques: SOE(Splicing by overlap extension) PCR

A. Primary PCR reaction

Segment1-smtBOP

primers

F

5' CGCGGATCCCTAGCGACACTCTTGTAAGTGA 3'

R

5' TTTAGCGATCACACTCATGACAGCAACTCCTTTGA 3'

PCR system (50ul)

parameters

procedure

temperature

time

pfu

0.5ul

PreDenature

94 ℃

2 min

primer F

2ul

Denature

94 ℃

30 sec

primer R

2ul

Annealing

53 ℃

30 sec

smt locus(PCR product)
diluted 100×

3ul

Extension

72 ℃

30 sec

dNTPs

8ul

Final Elongation

72 ℃

5 min

buffer

10ul

Final Hold

16 ℃

H2O

24.5ul

Cycle

30 cycles

Segment2-amilCP(BBa_K592009) or RFP(BBa_E1010)

primers

amilCP

F

5' GGAGTTGCTGTCATGAGTGTGATCGCTAAACAAATG 3'

R

5' CCGGAATTCTTATTAGGCGACCACAGGTT 3'

RFP

F

5' GGAGTTGCTGTCATGGCTTCCTCCGAAGACG 3'

R

5' CCGGAATTCGCGATCTACACTAGCACTATCAG 3'

PCR system (50ul)

parameters

procedure

temperature

time

pfu

0.5ul

PreDenature

94 ℃

2 min

primer F

2ul

Denature

94 ℃

30 sec

primer R

2ul

Annealing

53 ℃

30 sec

registered parts
diluted 100×

3ul

Extension

72 ℃

1 min

dNTPs

8ul

Final Elongation

72 ℃

5 min

buffer

10ul

Final Hold

16 ℃

H2O

24.5ul

Cycle

30 cycles

Fig.2 PCR product of primary reaction: 1. Marker (DL2000); 2, 3. amilCP(669bp); 6,7. RFP(708bp); 4, 5, 8 and 9. BOP(469bp)

Gel Extraction with TIANgel Midi Purification Kit(TIANGEN BIOTECH) see protocol

B. Overlapping and elongation

PCR system (50ul)

parameters

procedure

temperature

time

pfu

0.5ul

PreDenature

94 ℃

2 min

primer F&R

0ul

Denature

94 ℃

30 sec

segment 1

31.5ul in total
(mole number of segment
1 and 2=1:1)

Annealing

55 ℃

30 sec

segment 2

Extension

72 ℃

1 min

H2O

Final Elongation

72 ℃

5 min

dNTPs

8ul

Final Hold

16 ℃

buffer

10ul

Cycle

10 cycles

Fig.3 separation gel of step B 1. Marker (DL2000); 2. mixture containing BCP; 3. mixture containing BRP; the left arrow points at BCP; the right arrow points at BRP

Gel Extraction with TIANgel Midi Purification Kit(TIANGEN BIOTECH)

C. Second PCR reaction

primers

F

5' CGCGGATCCCTAGCGACACTCTTGTAAGTGA 3'

R

amilCP

5' CCGGAATTCTTATTAGGCGACCACAGGTT 3'

RFP

5' CCGGAATTCGCGATCTACACTAGCACTATCAG 3'

PCR system (50ul)

parameters

procedure

temperature

time

premix taq(TaKaRa)

25ul

PreDenature

94 ℃

5 min

primer F

2ul

Denature

94 ℃

30 sec

primer R

2ul

Annealing

53 ℃

30 sec

purified B’s product
diluted 100×

1ul

Extension

72 ℃

1.5 min

dNTPs

included in premix

Final Elongation

72 ℃

10 min

buffer

Final Hold

16 ℃

H2O

20ul

Cycle

30 cycles

Fig.4 PCR product of second reaction: 1. Marker; 2.BCP(1138bp); 3.BRP(1177bp); Marker (DL2000)

Gel Extraction with TIANgel Midi Purification Kit(TIANGEN BIOTECH) Ligation and transformation with pEASY-T5 Zero Cloning Kit from TransGen Biotech. See protocol

The sequencing result is consistent with our designation.

OPA(smtO-P and smtA)

primers

F

5' TTGGCGCGCGAGCCAATCACGGTTTGTCC 3'

R

5' CCAATGCATTTAGCCGTGGCAGTTACAGC 3'

PCR system (50ul)

parameters

procedure

temperature

time

premix taq(TaKaRa)

25ul

PreDenature

94 ℃

2 min

primer F

2ul

Denature

94 ℃

30 sec

primer R

2ul

Annealing

59 ℃

30 sec

smt locus(PCR product)
diluted 100×

1ul

Extension

72 ℃

30 sec

dNTPs

included in premix

Final Elongation

72 ℃

5 min

buffer

Final Hold

16 ℃

H2O

20ul

Cycle

30 cycles

Fig.5 PCR product of OPA(271bp); Marker (DL2000)

Gel Extraction with TIANgel Midi Purification Kit(TIANGEN BIOTECH) Ligation and transformation with pEASY-T5 Zero Cloning Kit from TransGen Biotech. The sequencing result is consistent with our designation.

FC(Flocculation gene, CP25 and CDS7)show sequence

The flocculation gene was successfully cloned from Bacillussp. F2.

While CP25 and CDS7 and the backbone sequence adjacent to them was synthesized by BGI Tech.And they are inserted in pMV.

We also used SOE PCR to splice flocculation gene and the rest ones.

A. Primary PCR reaction

Segment1-flocculation gene

primers

F

5' GGAATTCCATATGATGAGTCTACTTGCTGTTTTGTTTT 3'

R

5'AAGGGGTTATGCTAGTTACGAATTCGAGCTC 3'

PCR system (50ul)

parameters

procedure

temperature

time

pfu

0.5ul

PreDenature

94 ℃

2 min

primer F

2ul

Denature

94 ℃

30 sec

primer R

2ul

Annealing

58 ℃

30 sec

Flocculation gene(PCR product)
diluted 100×

3ul

Extension

72 ℃

1.5 min

dNTPs

8ul

Final Elongation

72 ℃

10 min

buffer

10ul

Final Hold

16 ℃

H2O

24.5ul

Cycle

30 cycles

Segment2-including CP25 and CDS7

primers

F

5' GAGCTCGAATTCGTAACTAGCATAACCCCTT 3'

R

5' CCCAAGCTTTTATTAAATATCCGCATGTTCCG 3'

PCR system (50ul)

parameters

procedure

temperature

time

pfu

0.5ul

PreDenature

94 ℃

2 min

primer F

2ul

Denature

94 ℃

30 sec

primer R

2ul

Annealing

58 ℃

30 sec

synthesized fragment(plasmid)
diluted 100×

3ul

Extension

72 ℃

30 sec

dNTPs

8ul

Final Elongation

72 ℃

5 min

buffer

10ul

Final Hold

16 ℃

H2O

24.5ul

Cycle

30 cycles

Fig.6 PCR product of the flocculation gene(1038bp) (arrows); Marker (DL2000)

Fig.7 PCR product of segment2(containing CP25 and CDS7, 217bp in total); Marker (DL2000)

Gel Extraction with TIANgel Midi Purification Kit(TIANGEN BIOTECH)

B. Overlapping and elongation

PCR system (50ul)

parameters

procedure

temperature

time

pfu

0.5ul

PreDenature

94 ℃

2 min

primer F&R

0ul

Denature

94 ℃

30 sec

segment 1

31.5ul in total
(mole number of segment
1 and 2=1:1)

Annealing

60 ℃

30 sec

segment 2

Extension

72 ℃

1.5 min

H2O

Final Elongation

72 ℃

10 min

dNTPs

8ul

Final Hold

16 ℃

buffer

10ul

Cycle

10 cycles

Fig.8 seperation gel of step B arrow points at FC; Marker (DL2000)

Gel Extraction with TIANgel Midi Purification Kit(TIANGEN BIOTECH)

C. Second PCR reaction

primers

F

5' GGAATTCCATATGATGAGTCTACTTGCTGTTTTGTTTT 3'

R

5' CCCAAGCTTTTATTAAATATCCGCATGTTCCG 3'

PCR system (50ul)

parameters

procedure

temperature

time

premix taq(TaKaRa)

25ul

PreDenature

94 ℃

5 min

primer F

2ul

Denature

94 ℃

30 sec

primer R

2ul

Annealing

58 ℃

30 sec

purified B’s product
diluted 100×

1ul

Extension

72 ℃

1.5 min

dNTPs

included in premix

Final Elongation

72 ℃

10 min

buffer

Final Hold

16 ℃

H2O

20ul

Cycle

30 cycles

Fig.9 PCR product of second reaction: FC(1267bp); Marker (DL2000)

Gel Extraction with TIANgel Midi Purification Kit(TIANGEN BIOTECH)

Ligation and transformation with pEASY-T5 Zero Cloning Kit from TransGen Biotech. The sequencing result is consistent with our designation.

All designed fragments would be replicated by PCR when needed in plasmid construction.

Plasmid construction

1. pHY300PLK-BCP-OPA

Insert BCP

Miniprep (pHY300PLK without BCP and OPA; pEASY-T5 cloning vector with BCP or OPA) with TIANprep Mini Plasmid Kit.see protocol

Double digestion (NEB)

substrate

BamH I-HF

EcoR I-HF

Cutsmart

Buffer

H2O

total

temperature

time

pHY300PLK

30ul

3ul

3ul

10ul

54ul

100ul

37

16 h

PCR product

30ul

3ul

3ul

10ul

54ul

100ul

37

16 h

Ligation (TaKaRa DNA Ligation Kit Ver.2.1see manual)

Solution I

-plasmid- & -BCP-

total

temperature

time

5ul

5ul in total (see note)

10ul

16

30 min

Note:-plasmid-:-BCP-(mole number)=1:2~1:8

Transformation see protocol

Colony PCR

primers

F

5' CGCGGATCCCTAGCGACACTCTTGTAAGTGA 3'

R

5' CCGGAATTCTTATTAGGCGACCACAGGTT 3'

PCR system (20ul)

parameters

procedure

temperature

time

premix taq(TaKaRa)

10ul

PreDenature

94

5 min

primer F

0.8ul

Denature

94

30 sec

primer R

0.8ul

Annealing

53

30 sec

template: pick a single colony and dip in H2O

8.4ul

Extension

72

1.5 min

Final Elongation

72

10 min

dNTPs

included in premix

Final Hold

16

buffer

Cycle

30 cycles

Note: The template was heat denatured at 100 in metal bath, then freeze on ice for 2 min

before running through parameters on the right.

Fig.10 1. Marker (DL2000); 2-5. each for one single colony(all positive); 6. positive control; 7. H2O control

Miniprep (pHY300PLK with maybe BCP) with TIANprep Mini Plasmid Kit.as before Double digestion (NEB) for detection

Plasmids with H2O

BamH I-HF

EcoR I-HF

Cutsmart

Buffer

total

temperature

time

16.8ul

0.6ul

0.6ul

2ul

20ul

37

16 h

Fig.11 digestion detection: 1. digestion product of positive clone plasmid DNA; 2. linearized vector; 3. BCP; 4. Marker (DL15000)

The sequencing result is consistent with our designation.

Insert OPA

Miniprep (pHY300PLK with only BCP; pEASY-T5 cloning vector with OPA) with TIANprep Mini Plasmid Kit.

Two-step enzyme digestion(NEB)(total 100ul)

substrate

Nsi I

Buffer 3.1

H2O

temperature

time

BssH II

temperature

time

pHY300PLK-BCP

30ul

3ul

10ul

54ul

37

3 h

3ul

50

3 h

PCR product

30ul

3ul

10ul

54ul

37

3 h

3ul

50

3 h

Ligation (TaKaRa DNA Ligation Kit Ver.2.1 as before)

Solution I

-plasmid- & -OPA-

total

temperature

time

5ul

5ul in total (see note)

10ul

16

30 min

Note:-plasmid-:-OPA-(mole number)=1:2~1:8

Transformation

Colony PCR

primers

F

5' TTGGCGCGCGAGCCAATCACGGTTTGTCC 3'

R

5' CCAATGCATTTAGCCGTGGCAGTTACAGC 3'

PCR system (20ul)

parameters

procedure

temperature

time

premix taq(TaKaRa)

10ul

PreDenature

94 ℃

5 min

primer F

0.8ul

Denature

94 ℃

30 sec

primer R

0.8ul

Annealing

59 ℃

30 sec

template: pick a single colony and dip in H2O

8.4ul

Extension

72 ℃

30 sec

Final Elongation

72 ℃

5 min

dNTPs

included in premix

Final Hold

16 ℃

buffer

Cycle

30 cycles

Note: The template was heat denatured at 100℃ in metal bath, then freeze on ice for 2 min
before running through parameters on the right.

Fig.12 1-4. each for one single colony(all positive); 5.positive control; 6. H2O control; 7. Marker Miniprep (pHY300PLK with BCP and maybe OPA) with TIANprep Mini Plasmid Kit.

Two-step enzyme digestion(NEB) for detection

Plasmids with H2O

Nsi I

Buffer 3.1

temperature

time

BssH II

temperature

time

total

16.8ul

0.6ul

2ul

37℃

3 h

0.6ul

50℃

3 h

20ul

Fig.13 digestion detection: 1. Marker (DL5000); 2. digestion product of positive clone plasmid DNA; 3. linearized vector; 4. OPA

The sequencing result is consistent with our designation.

2. pHY300PLK-BRP-OPA

Insert BRP

Miniprep (pHY300PLK without BRP and OPA; pEASY-T5 cloning vector with BRP) with TIANprep Mini Plasmid Kit.

Double digestion (NEB)

substrate

BamH I-HF

EcoR I-HF

Cutsmart
Buffer

H2O

total

temperature

time

pHY300PLK

30ul

3ul

3ul

10ul

54ul

100ul

37℃

16 h

PCR product

30ul

3ul

3ul

10ul

54ul

100ul

37℃

16 h

Ligation (TaKaRa DNA Ligation Kit Ver.2.1 as before)

Solution I

-plasmid- & -BRP-

total

temperature

time

5ul

5ul in total (see note)

10ul

16℃

30 min

Note:-plasmid-:-BRP-(mole number)=1:2~1:8

Transformation

Colony PCR

primers

F

5' CGCGGATCCCTAGCGACACTCTTGTAAGTGA 3'

R

5' CCGGAATTCGCGATCTACACTAGCACTATCAG 3'

PCR system (20ul)

parameters

procedure

temperature

time

premix taq(TaKaRa)

10ul

PreDenature

94 ℃

5 min

primer F

0.8ul

Denature

94 ℃

30 sec

primer R

0.8ul

Annealing

53 ℃

30 sec

template: pick a single colony and dip in H2O

8.4ul

Extension

72 ℃

1.5 min

Final Elongation

72 ℃

10 min

dNTPs

included in premix

Final Hold

16 ℃

buffer

Cycle

30 cycles

Note: The template was heat denatured at 100℃ in metal bath, then freeze on ice for 2 min
before running through parameters on the right.

Fig.14 1. Marker (DL2000); 2-5. each for one single colony(all positive); 6.H2O control; 7. positive control

Miniprep (pHY300PLK with maybe BRP) with TIANprep Mini Plasmid Kit.

Double digestion (NEB) for detection

Plasmids with H2O

BamH I-HF

EcoR I-HF

Cutsmart 

Buffer

total

temperature

time

16.8ul

0.6ul

0.6ul

2ul

20ul

37

16 h

Fig.15 digestion detection: 1. Marker (DL15000); 3. digestion product of positive clone plasmid DNA

The sequencing result is consistent with our designation.

Insert OPA

Miniprep (pHY300PLK with only BRP; pEASY-T5 cloning vector with OPA) with TIANprep Mini Plasmid Kit.

Two-step enzyme digestion(NEB)(total 100ul)

substrate

Nsi I

Buffer 3.1

H2O

temperature

time

BssH II

temperature

time

pHY300PLK-BRP

30ul

3ul

10ul

54ul

37

3 h

3ul

50

3 h

PCR product

30ul

3ul

10ul

54ul

37

3 h

3ul

50

3 h

Ligation (TaKaRa DNA Ligation Kit Ver.2.1 as before)

Solution I

-plasmid- & -OPA-

total

temperature

time

5ul

5ul in total (see note)

10ul

16

30 min

Note:-plasmid-:-OPA-(mole number)=1:2~1:8

Transformation

Colony PCR

primers

F

5' TTGGCGCGCGAGCCAATCACGGTTTGTCC 3'

R

5' CCAATGCATTTAGCCGTGGCAGTTACAGC 3'

PCR system (20ul)

parameters

procedure

temperature

time

premix taq(TaKaRa)

10ul

PreDenature

94 

5 min

primer F

0.8ul

Denature

94 

30 sec

primer R

0.8ul

Annealing

59 

30 sec

template: pick a single colony and dip in H2O

8.4ul

Extension

72 

30 sec

Final Elongation

72 

5 min

dNTPs

included in premix

Final Hold

16 

buffer

Cycle

30 cycles

Note: The template was heat denatured at 100℃ in metal bath, then freeze on ice for 2 min 

before running through parameters on the right.

Fig.16 1. Marker (DL2000); 2-15. each for one single colony(8 positive); 16. H2O control; 17. positive control

Miniprep (pHY300PLK with BRP and maybe OPA) with TIANprep Mini Plasmid Kit.

Two-step enzyme digestion(NEB) for detection

Plasmids with H2O

Nsi I

Buffer 3.1

temperature

time

BssH II

temperature

time

total

16.8ul

0.6ul

2ul

37

3 h

0.6ul

50

3 h

20ul

Fig.17 digestion detection: 1. Marker (DL5000); 2. digestion product of positive clone plasmid DNA; 3. linearized vector; 4. OPA

The sequencing result is consistent with our designation.

3. PACYC184-BCP-OPA

Insert OPA

Miniprep (pACYC184 without BCP and OPA; pEASY-T5 cloning vector with OPA) with TIANprep Mini Plasmid Kit.

Single enzyme digestion (TaKaRa)

substrate

Xba I

0.1% BSA

10×M

Buffer

H2O

total

temperature

time

pACYC184

30ul

3ul

10ul

10ul

47ul

100ul

37

16 h

PCR product

30ul

3ul

10ul

10ul

47ul

100ul

37

16 h

Ligation (TaKaRa DNA Ligation Kit Ver.2.1 as before)

Solution I

-plasmid- & -OPA-

total

temperature

time

5ul

5ul in total (see note)

10ul

16

30 min

Note:-plasmid-:-OPA-(mole number)=1:2~1:8

Transformation

Colony PCR

primers

F

5' TGCTCTAGAGAGCCAATCACGGTTTGTCC 3'

R

5' TGCTCTAGATTAGCCGTGGCAGTTACAGC 3'

PCR system (20ul)

parameters

procedure

temperature

time

premix taq(TaKaRa)

10ul

PreDenature

94

5 min

primer F

0.8ul

Denature

94

30 sec

primer R

0.8ul

Annealing

59

30 sec

template: pick a single colony and dip in H2O

8.4ul

Extension

72

30 sec

Final Elongation

72

5 min

dNTPs

included in premix

Final Hold

16

buffer

Cycle

30 cycles

Note: The template was heat denatured at 100 in metal bath, then freeze on ice for 2 min

before running through parameters on the right.

Fig.18 1-6. each for one single colony(1,4,6 negative; 2,3,5 positive); 7.positive control; 8. H2O control; 9. Marker

Miniprep (pACYC184 with maybe OPA) with TIANprep Mini Plasmid Kit.

Single enzyme digestion (TaKaRa) for detection

Plasmids with H2O

Xba II

0.1% BSA

10×M

Buffer

total

temperature

time

15.75ul

0.25ul

2ul

2ul

20ul

37

16 h

Fig.19 digestion detection: 1. 15000bp marker 2-5. digestion product of positive clone plasmid DNA; 6. 2000bp marker; the upper arrow points at linearization vector; the lower arrow points at OPA

The sequencing result is consistent with our designation.

Insert BCP

Miniprep (pACYC184 with only OPA; pEASY-T5 cloning vector with BCP) with TIANprep Mini Plasmid Kit. as before

Single enzyme digestion (TaKaRa)

substrate

Sac II

0.1% BSA

10×T

Buffer

H2O

total

temperature

time

pACYC184-OPA

30ul

3ul

10ul

10ul

47ul

100ul

37

16 h

PCR product

30ul

3ul

10ul

10ul

47ul

100ul

37

16 h

Ligation (TaKaRa DNA Ligation Kit Ver.2.1 as before)

Solution I

-plasmid- & -BCP-

total

temperature

time

5ul

5ul in total (see note)

10ul

16

30 min

Note:-plasmid-:-BCP-(mole number)=1:2~1:8

Transformation

Colony PCR

primers

F

5' TCCCCGCGGCTAGCGACACTCTTGTAAGTGA 3'

R

5' TCCCCGCGGTTATTAGGCGACCACAGGTT 3'

PCR system (20ul)

parameters

procedure

temperature

time

premix taq(TaKaRa)

10ul

PreDenature

94

5 min

primer F

0.8ul

Denature

94

30 sec

primer R

0.8ul

Annealing

58

30 sec

template: pick a single colony and dip in H2O

8.4ul

Extension

72

1.5 min

Final Elongation

72

10 min

dNTPs

included in premix

Final Hold

16

buffer

Cycle

30 cycles

Note: The template was heat denatured at 100 in metal bath, then freeze on ice for 2 min

before running through parameters on the right.

Fig.20 1. Marker (DL2000); 2. H2O control; 3-13. each for one single colony (3-11 negative; 12, 13 positive); 14. positive control

Miniprep (pACYC184 with OPA and maybe BCP) with TIANprep Mini Plasmid Kit. as before

Single digestion(TaKaRa) for detection

Plasmids with H2O

Sac II

0.1% BSA

10×T

Buffer

total

temperature

time

15.75ul

0.25ul

2ul

2ul

20ul

37

16 h

Fig.21 digestion detection: 1. Marker (DL5000) 2. digestion product of positive clone plasmid DNA; 3. linearized vector; 4. BCP

The sequencing result is consistent with our designation.

4.PACYC184-BRP-OPA

Insert BRP

Miniprep (pACYC184 with only OPA; pEASY-T5 cloning vector with BRP) with TIANprep

Mini Plasmid Kit.

Single enzyme digestion (TaKaRa)

substrate

Sac II

0.1% BSA

10×T

Buffer

H2O

total

temperature

time

pACYC184-OPA

30ul

3ul

10ul

10ul

47ul

100ul

37

16 h

PCR product

30ul

3ul

10ul

10ul

47ul

100ul

37

16 h

Ligation (TaKaRa DNA Ligation Kit Ver.2.1 as before)

Solution I

-plasmid- & -BRP-

total

temperature

time

5ul

5ul in total (see note)

10ul

16

30 min

Note:-plasmid-:-BCP-(mole number)=1:2~1:8

Transformation

Colony PCR

primers

F

5' TCCCCGCGGCTAGCGACACTCTTGTAAGTGA 3'

R

5' TCCCCGCGGGCGATCTACACTAGCACTATCAG 3'

PCR system (20ul)

parameters

procedure

temperature

time

premix taq(TaKaRa)

10ul

PreDenature

94

5 min

primer F

0.8ul

Denature

94

30 sec

primer R

0.8ul

Annealing

53

30 sec

template: pick a single colony and dip in H2O

8.4ul

Extension

72

1.5 min

Final Elongation

72

10 min

dNTPs

included in premix

Final Hold

16

buffer

Cycle

30 cycles

Note: The template was heat denatured at 100 in metal bath, then freeze on ice for 2 min

before running through parameters on the right.

Fig.22 1. Marker (DL2000); 2-4. each for one single colony (4 positive); 5. positve control; 6. H2O control

Miniprep (pACYC184 with OPA and maybe BRP) with TIANprep Mini Plasmid Kit.

Single digestion(TaKaRa) for detection

Plasmids with H2O

Sac II

0.1% BSA

10×T  Buffer

total

temperature

time

15.75ul

0.25ul

2ul

2ul

20ul

37

16 h

Fig.23 digestion detection: the upper arrow points at linearization vector; the lower arrow points at BRP The sequencing result is consistent with our designation. Marker (DL2000)

5.pET-28b(+)-Flo-CDS7

Miniprep (pET-28b(+) without FC; pEASY-T5 cloning vector with FC) with TIANprep Mini Plasmid Kit.

Double digestion (NEB)

substrate

Hind III-HF

Nde I

Cutsmart

Buffer

H2O

total

temperature

time

pET-28b(+)

30ul

3ul

3ul

10ul

54ul

100ul

37

16 h

PCR product

30ul

3ul

3ul

10ul

54ul

100ul

37

16 h

Ligation (TaKaRa DNA Ligation Kit Ver.2.1 as before)

Solution I

-plasmid- & -FC-

total

temperature

time

5ul

5ul in total (see note)

10ul

16

30 min

Note:-plasmid-:-FC-(mole number)=1:2~1:8

Transformation

Colony PCR

primers

F

5' GGAATTCCATATGATGAGTCTACTTGCTGTTTTGTTTT 3'

R

5' CCCAAGCTTTTATTAAATATCCGCATGTTCCG 3'

PCR system (20ul)

parameters

procedure

temperature

time

premix taq(TaKaRa)

10ul

PreDenature

94

5 min

primer F

0.8ul

Denature

94

30 sec

primer R

0.8ul

Annealing

58

30 sec

template: pick a single colony and dip in H2O

8.4ul

Extension

72

1.5 min

Final Elongation

72

10 min

dNTPs

included in premix

Final Hold

16

buffer

Cycle

30 cycles

Note: The template was heat denatured at 100 in metal bath, then freeze on ice for 2 min

before running through parameters on the right.

Fig.23 1-5. each for one single colony(all positive); 6.positive control; 7. H2O control; 8. Marker (DL2000)

Miniprep (pET-28b(+) with maybe FC) with TIANprep Mini Plasmid Kit. Double digestion (NEB) for detection

Plasmids with H2O

Hind III-HF

Nde I

Cutsmart

Buffer

total

temperature

time

16.8ul

0.6ul

0.6ul

2ul

20ul

37

16 h

Fig.25 digestion detection: 1. 2000bp marker; 3. negative result for worse digestion; 4-6. pET-14b(++) vector; 7. 15000bp marker

The sequencing result is consistent with our designation.

Protein characterization

Protein characterization by SDS-PAGE. see protocol

Fig.26 result of SDS-PAGE 1,2,3. Analysis of amilCP; 5,6,7. Annalysis of RFP; 1&5. not induced; 2&6. Proteins from IPTG induced(0.8mM) E.coli.; 3&7. Control without reporter gene; 4. Protein marker