Click Chemistry - Jena Bioscience · 2017. 11. 2. · Jena BioscienceGmbH LöbstedterStr. 71 07749...

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Jena Bioscience GmbH Löbstedter Str. 71 07749 Jena, Germany Tel.: +49-3641-628-5000 Fax: +49-3641-628-5100 Web: www.jenabioscience.com Jena, October 24 th 2017 Click Chemistry – Expanding the Scope of Nucleic Acid Labeling Logo Client

Transcript of Click Chemistry - Jena Bioscience · 2017. 11. 2. · Jena BioscienceGmbH LöbstedterStr. 71 07749...

Page 1: Click Chemistry - Jena Bioscience · 2017. 11. 2. · Jena BioscienceGmbH LöbstedterStr. 71 07749 Jena, Germany Tel.: +49-3641-628-5000 Fax: +49-3641-628-5100 Web: Jena, October24th

Jena Bioscience GmbHLöbstedter Str. 7107749 Jena, Germany

Tel.: +49-3641-628-5000Fax: +49-3641-628-5100Web: www.jenabioscience.com

Jena, October 24th 2017

Click Chemistry –Expanding the Scope of Nucleic Acid Labeling

Logo Client

Page 2: Click Chemistry - Jena Bioscience · 2017. 11. 2. · Jena BioscienceGmbH LöbstedterStr. 71 07749 Jena, Germany Tel.: +49-3641-628-5000 Fax: +49-3641-628-5100 Web: Jena, October24th

Click Chemistry on Nucleic Acids

1. Definition and Hallmarks of a Click Reaction

2. Classification of Click Reactions

3. In vitro Synthesis of DNA and RNA Conjugates

4. Clickable Nucleosides in Metabolic Labeling

5. Trends and Perspectives

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“Diverse Function from a Few Good Reactions“[1]

§ Selective: Formation of only the desired

product

§ Orthogonal: No side reaction with sample matrix

§ Simple: Easy to do for a non-chemist

§ Fast: Completion in biomolecular timescale

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K. Barry SharplessNoble Price Chemistry 2001

A + B A BClick?

[1] Kolb et al. (2001) Angew. Chem. Int. Ed. Engl. 40(11): 2004

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[1] Rostovtsev et al. (2002) Angew. Chem. Int. Ed. Engl. 41(14):2596[2] Tornøe et al. (2002) J. Org. Chem. 67(9):3057[3] Agard et al. (2004) JACS. 126(46):15046

Azide Clicks with Alkyne in the Presence of Cu(I) or throughRing Strain

A B+Cu(I)

(CuAAC)

Alkyne-containingmolecule A

Azide-containingmolecule B

Conjugate of A and B, cross-linked via a Triazole moiety

AB

NNN

NNN

N

O

N

ONN

N

AB

Azide-containingmolecule B

NNN

DBCO-containingmolecule A

A

B+ SPAAC

N

NNN

N NN

NNN

HOO

N

NNN

N NN

NNN

HOHO

OHTHPTA BTTAA

• CuSO4, reduced in situ• Ascorbate

Cu(I)-stabilizingLigands

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Tetrazines Click with Alkenes

A

Tetrazine-functionalizedmolecule A

+Vinyl-

functionalizedmolecule B

B

NN N

N

R2

R1

B

A

NNH

R2

R1

Conjugate of A and B crosslinkedvia Dihydropyrazine

B+

Methylcyclopropene-functionalized

molecule B

B+

trans-Cyclooctene(TCO)-

functionalizedmolecule B

B

A

NNH

R2

R1

A

BNNH

R2

R1

Carboni and Lindsey (1959) JACS 81(16):4342.5

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How Fast is Fast Enough?

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A + B A Bk2

NHR

O

NN N

N

R1

R2

+N

NN

+

N

O

NNN

+

M-1s-1

Isolated Material Fixed Cells/Life Cell Surface Life Cells Cytosol

10-3 10-2 10 102 106

NH

O

ONO

OH

HON O

O

N O

O

+

NN N

N

R1

R2

+

NN N

N

R1

R2

[1] Oliveira et al. (2017) Chem. Soc. Rev. 46(16):4895[2] Kozma et al. (2017) ChemBioChem. 18(6):486

Slow Fast

Page 7: Click Chemistry - Jena Bioscience · 2017. 11. 2. · Jena BioscienceGmbH LöbstedterStr. 71 07749 Jena, Germany Tel.: +49-3641-628-5000 Fax: +49-3641-628-5100 Web: Jena, October24th

Click Chemistry on Nucleic Acids

1. Definition and Hallmarks of a Click Reaction

2. Classification of Click Reactions

3. In vitro Synthesis of DNA and RNA Conjugates

4. Clickable Nucleosides in Metabolic Labeling

5. Trends and Perspectives

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Dual DNA Labeling for FRET and TIRF in One Pot

§ CuAAC (and SPAAC) are orthogonal to iEDDA

§ Single step/ one pot procedure for DNA labeling

§ è Easy combination of diverse labels

§ è No de novo synthesis of DNA required

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CuSO4,THPTA

Ascorbate

[1] Schoch et al. (2012) Bioconjug. Chem. 23(7):1382

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Polymerases:Pwo,Vent (exo-)KOD XL

Internal Modification of Long DNA by Incorporation ofFunctionalized dNTPs

§ Tolerance of most DNA-polymerases towards modified dNTPs

§ C-5-modification of dU/dC particularly well suited (major groove)

§ Variable degree of substitution by adjusting dNTP/dNTP*

§ Modified amplicons of several kb accessible

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[1] Burley et al. (2006) JACS 128 (5):1398[2] Gierlich et al. (2007) Chem. - Eur. J. 13 (34):9486

NH 3

2NH1

6

5 4

O

7O

8

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Efficient Synthesis and KOD XL- Incorporation of 5-N3-dCTP

10[1] Krause et al. (2014) Chem. - Eur. J. 20(50): 16613

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Preparing RNAs beyond the Scope of Solid Phase Synthesis

§ C5-modified UTP derivatives are substrates of the T7-RNA polymerase

§ Generally, fewer polymerases available than for DNA/PCR

§ Synthesis of several kb transcripts possible in vitro

§ Constraints apply due to conserved promoter sequences

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[1] Rao et al. (2012) Chem. Commun. (Camb). 48(4):498[2] Sawant et al. (2016) Nucleic Acids Res. 44(2):e16

Sawant et al. (2016) Nucleic Acids Res. 44(2):e16

NH

O

ONO

OHOH

OPOOH

OPOPHOOO

OHOH

N3

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Chemo-Enzymatic 3′- and Internal RNA Modification UsingPolyA-polymerases and Ligases

§ Limited accessibility of long internally modified RNA by chemical means

§ Chemo-enzymatic approaches to overcome synthetic limitation

§ Azides are small

12[1] Winz et al. (2012) Nucleic Acids Res. 40(10):e78

Page 13: Click Chemistry - Jena Bioscience · 2017. 11. 2. · Jena BioscienceGmbH LöbstedterStr. 71 07749 Jena, Germany Tel.: +49-3641-628-5000 Fax: +49-3641-628-5100 Web: Jena, October24th

Chemo-Enzymatic 3′- and Internal RNA Modification UsingPolyA-polymerases and Ligases

13[1] Winz et al. (2012) Nucleic Acids Res. 40(10):e78

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Partially Complementary DNA Scaffolds Increase Click Yields

§ Increasing the efficiency of CuAAC on internal azide

§ Forcing the ligation site into a bulge

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75-85% without scaffold92% with scaffold

[1] Winz et al. (2012) Nucleic Acids Res. 40(10):e78

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TdT permits 3′- and Internal Modification of DNA byTailing and Extension

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§ Transfer of various base-modified (d)NTPs by

terminal deoxynucleotidyl transferase TdT

§ Fill-up by polymerase or enzymatic ligation

[1] Winz et al. (2015) Nucleic Acids Res. 43(17): e110

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T7 RNAP

SP6 RNAP

T3 RNAP

5-(d)UpG Dinucleotides Are Excellent Transcriptional Initiators

§ (d)UpGs are universally applicable

16[1] Samanta et al. (2014) Chem Commun. 50(11):1313

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dUpG-Priming Allows to Decorate RNA with Metal Complexes, Affinity Tags, Sugars, Surfactants, Dyes, …

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A

B

C

[1] Samanta et al. (2014) Chem Commun. 50(11):1313

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The 5′-OdUpG Label is a Ligation Donor for Internalization

§ Requirements of ligation approach:

§ Acceptance by polynucleotide kinase

§ Acceptance by ligases

§ 5-UpG modification tolerated bythree different enzyme classes

§ Two-step procedure

18[1] Samanta et al. (2014) Chem Commun. 50(11):1313

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Chemo-Enzymatic Procedures Are Applicable to Any Positionin Any Nucleic Acid

InternalRandom Site-Specific

3′ 5′

DNA

RNA

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Click Chemistry on Nucleic Acids

1. Definition and Hallmarks of a Click Reaction

2. Classification of Click Reactions

3. In vitro Synthesis of DNA and RNA Conjugates

4. Clickable Nucleosides in Metabolic Labeling

5. Trends and Perspectives

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Cytoplasm

Nucleus

Base Base Phosphorylation ofnucleoside analog by

cellular kinases

In vivo Application of Clickable Nucleosides: Metabolic Labels

DNAP

A Replication

RNAP

B Transcription

PAP

C Polyadenylation

NH

O

ONO

OH

HO

NH

O

ONO

OH

HO

NH

O

ONO

OH

HO

N3N

NH2

ONO

OH

HO

NH

O

ONO

OH

HO F

[1] Salic and Mitchison (2008) PNAS 105 (7):2415[2] Neef and Luedtke (2011) PNAS 108(51): 20404[3] Guan et al. (2011) ChemBioChem 2 (14):2184[4] Neef and Luedtke (2011) Chembiochem. 15(6):789[5] Rieder and Luedtke (2014) Angew. Chem. Int. Ed. Engl. 53(35):9168[6] Jao and Salic (2008) PNAS 105(41): 15779[7] Curanovic et al. (2013) Nat. Chem. Biol. 9 (11):671 21

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Click Chemistry Permits Direct Introduction ofAffinity Tags

§ Analysis of mRNA-polyadenylation

§ Biotin tag ideally suited for streptavidin pulldown and NGS22

Feeding

N

NN

NNH2

O

OHOH

HO

Lysis/ RNA-isolation

CuAAC

Biotin-N3N

NN

S

NHHN

O

Agarose GelSeparation

Northern-Blot

Strep-AP

LuminescenceDetection

Curanovic et al. (2013) Nat. Chem. Biol. 9 (11):671

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Superior Efficiency of Click-Labeling to Immunostaining

§ No Antibodies required

§ Label can easily be adapted to individual needs

§ Mutual orthogonality of both techniques23

FixationFeeding

NH

O

ONO

OH

HO

Br

Yanti-Br

BrBrBr

BrBrBr

BrBrBr

Yanti-Fc

BrBrBr

Y

A

NH

O

ONO

OH

HO

N3

FixationFeeding Click

B

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Visualization of Metabolically Labeled DNA and RNA

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Salic and Mitchison (2008) PNAS 105 (7):2415

NH

O

ONO

OH

HO

Rieder and Luedtke (2014) Angew. Chem. Int. Ed. Engl. 53(35): 9168

NH

O

ONO

OH

HO F

NH

O

ONO

OH

HO

NH

O

ONO

OH

HO

Br

Jao and Salic (2008) PNAS 105(41): 15779

NH

O

ONO

OHOH

HO

Page 25: Click Chemistry - Jena Bioscience · 2017. 11. 2. · Jena BioscienceGmbH LöbstedterStr. 71 07749 Jena, Germany Tel.: +49-3641-628-5000 Fax: +49-3641-628-5100 Web: Jena, October24th

Click Chemistry on Nucleic Acids

1. Definition and Hallmarks of a Click Reaction

2. Classification of Click Reactions

3. In vitro Synthesis of DNA and RNA Conjugates

4. Clickable Nucleosides in Metabolic Labeling

5. Trends and Perspectives

25

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The (Last) Challenge Remaining- Life Cell Imaging

§ Already well established in protein science

§ Metabolic nucleotide labels are rather slow

§ Cytotoxicity of copper

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[1] Carlson et al. (2013) Angew. Chem. Int. Ed., 52(27): 6917[2] Uttamapinant et al. (2012). Angew. Chem. Int. Ed. Engl. 51 (24):5852.

N B- N+

FF

NN

NN

R

+N B- N

+

FF

NHN

R

OHOH

1600 x turn-on

Turn-On-Tetrazines[1]

N

O

NH

NN N

Cu+

R+N

O

NH N

NNR

10 x decreasedCu(I)-demand

Picolyl Azides[2]

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Click Chemistry Is Useful for Anybody Dealing withNucleic Acid Analytics

§ Click reactions are broadly applicable to nucleic acids

§ High modularity in experimental design

§ Small tags are well tolerated by various enzyme classes

§ Allow preparation of previously inaccessible conjugates

§ Virtually any click precursor commercially available

§ Life cell applications subject to current research

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40 People…

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…working at our new 2,500 m2 corporate building