Global Sales Review September 2008

NEB Competent Cell Product Portfolio February 2013 Global Sales Review September 2008 Jim Samuelson Gene Expression Division

The NEB Competent Cell Product Portfolio For Protein Expression NEB Express NEB Express Iq T7 Express T7 Express Iq T7 Express lysY/Iq T7 Express lysY T7 Express Crystal Shuffle Express Shuffle T7 Express Shuffle T7 Express lysY Shuffle T7 For Cloning/ Plasmid Isolation NEB 10-beta NEB 5-alpha NEB 5-alpha Iq NEB Turbo dam-/dcm- BL21 BL21(DE3) Lemo21(DE3) NiCo21(DE3)

Cloning strain vs. Protein expression strain • Cloning strain • Essential: High transformation efficiency (>1 x 109) • endA1 Activity of nonspecific endonuclease I is eliminated • for high quality plasmid preparations • Desirable: recA1 Reduced recombination of cloned DNA • Protein expression strain • Desirable: protease deficient (e.g. Lon, OmpT) • endA1(all “Express” strains carry this mutation) • lacIqand/or lysY function to control basal protein expression

Strains For Cloning and Plasmid Isolation NEB 10-beta NEB 5-alpha NEB 5-alpha Iq NEB Turbo dam-/dcm-

C3019H/I C3020K NEB 10-beta Competent E. coli • * DH10B™ equivalent • * rapid growth recA strain (reduced recombination of cloned DNA) • * transformation of large plasmids and BACs (greater than 10kb) • * Activity of nonspecific endonuclease I (endA1) eliminated for highest quality plasmid preparations • * Efficient transformation of methylated DNA derived from eukaryotic sources or unmethylated DNA derived from PCR, cDNA and many other sources [mcrAΔ(mrr-hsdRMS-mcrBC)] • * Resistance to phage T1 (fhuA2) • * Suitable for blue/white screening with cloning vectors expressing the lacZα peptide • (No IPTG required if plasmid does not encode the lacI gene, only X-gal required) • * K12 Strain

C2987H/I C2989K NEB 5-alpha Competent E. coli * DH5α™ equivalent * Reduced recombination of cloned DNA (recA1) * Activity of endonuclease I (endA1) eliminated for highest quality plasmid preparations * Free of animal products * Efficient transformation of unmethylated DNA derived from PCR, cDNA and many other sources (hsdR) * Resistance to phage T1 (fhuA2) * Suitable for blue/white screening with cloning vectors expressing the lacZα peptide * K12 Strain

NEB 5-alpha IqCompetent E. coli C2992H/I * DH5α™ equivalent * Tight control of expression by laclq allows potentially toxic genes to be cloned * Reduced recombination of cloned DNA (recA1) * Activity of endonuclease I (endA1) eliminated for highest quality plasmid preparations * Free of animal products * Efficient transformation of unmethylated DNA derived from PCR, cDNA and many other sources (hsdR) * Resistance to phage T1 (fhuA2) * Suitable for blue/white screening with cloning vectors expressing the lacZα peptide * K12 Strain

C2984H/I C2986K NEB Turbo Competent E. coli • * Highest growth rate on agar plates - visible colonies 6.5 hours after transformation • * Isolate DNA after 4 hours of culturing a single overnight colony • * Tight control of expression by laclq allows potentially toxic genes to be cloned • * Activity of endonuclease I (endA1) eliminated for highest quality plasmid preparations • * Resistance to phage T1 (fhuA2) • * Suitable for blue/white screening with cloning vectors expressing the lacZα peptide • * Suitable for 5 minute transformation protocol with AmpR plasmids • * EcoKr-m-, McrBC- • * K12 Strain

NEB Turbo – The Fastest Growing Competent Cells Available • Colonies visible after just 6.5 h. • Available as chemical or electrocompetent cells.

NEB Turbo is recA+ • When should this be a concern during cloning experiments? • Cloning vector contains regions of homology to the E. coli chromosome • Cloned DNA fragment contains homology to the E.coli chromosome • Cloned DNA fragment contains repeat elements • Undesired clone recombination is more likely with high-copy vectors • e.g. pUC origin of replication • pUC copy number may be reduced by reducing the growth temperature

Cloning/ propagation of unstable DNA Current recommendation is NEB-10beta Reduce plating and culture temperature to reduce plasmid copy number

C2925H dam-/dcm-Competent E. coli • * Dam and Dcm methylation (shown below) is not present in the dam-/dcm-strain • 5’-GATC-3’ 5’-CCWGG-3’ • 3’-CTAG-5’ 3’-GGWCC-5’ • * Activity of nonspecific endonuclease I (endA1) eliminated for highest quality plasmid preparations • * T1 phage resistant (fhuA2) • * K12 Strain Note: strain is resistant to chloramphenicol m m m m

Protein Expression strains BL21(DE3) Lemo21(DE3) NiCo21(DE3) BL21 NEB Express NEB Express Iq T7 Express T7 Express Iq T7 Express lysY/Iq T7 Express lysY T7 Express Crystal Shuffle Express Shuffle T7 Express Shuffle T7 Express lysY Shuffle T7 also B strains Notes: “Express” indicates a B strain “T7” or “DE3” indicates compatibility with T7 promoter vectors K-12 strain

NEB Express, NEB Express Iq or BL21 C3037 C2530 C2523 • * Deficient in proteases Lon and OmpT • * Do not express the T7 RNA polymerase Applications: protein expression from lac, tac, trc, and araBAD promoters recommended strains for pMAL expression of MBP fusion proteins NEB Express Iq is especially useful for protein expression from vectors without the lacI gene Note:NEB Express Iq is resistant to chloramphenicol

Vector – protein expression strain compatibility

BL21(DE3) The most commonly used protein expression strain gene1 = phage T7 RNA polymerase gene UV5 = lacUV5 promoter, repressed by LacI protein induced by IPTG

Comparison: BL21(DE3) vs. T7 Express strains BL21(DE3) is truly difficult to make chemically competent T7 Express strains offer approx. 100-fold higher transformation efficiency BL21(DE3) expresses endonuclease I – direct cloning is not advised T7 Express strains are endA1 - direct cloning is an option, isolated plasmid is clean enough for sequencing BL21(DE3)-protein expression from T7 promoters is not tightly controlled

T7 expression is not tightly controlled in BL21(DE3) Remedy: co-expression of T7 lysozyme, the natural inhibitor of T7 RNA polymerase BL21(DE3) pLysS = moderate expression of wt T7 lysozyme BL21(DE3) pLysE = high expression of wt T7 lysozyme T7 Express lysY and T7 Express lysY/Iq Expression of K128Y variant of T7 lysozyme

Strict control of T7 expression in lysY strains Remedy: co-expression of T7 lysozyme, the natural inhibitor of T7 RNA polymerase lysY is the K128Y variant of T7 lysozyme • controls T7 RNA polymerase expression of protein • Cell envelope integrity is not • compromised (no amidase activity) • lysY is carried by a single-copy mini-F plasmid in T7 Express strains • Antibiotic selection is not necessary Zn K128Y Cheng et al. Proc. Natl. Acad. Sci., USA (1994)

Comparison: BL21(DE3) vs. T7 Express strains Non-toxic protein expression minus/ plus inducer Toxic clone transformation IPTG

T7 Express Crystal Competent E. coli (High Efficiency) C3022H/I Designed for seleno-methionine labeling of proteins for x-ray crystallography studies metB1 mutation allows user to dictate the level of seleno-methionine incorporation NotI x-ray diffraction pattern NotI crystal

Lemo21(DE3) ”Less is more” periplasm outer membrane inner membrane cytoplasm The superior T7 strain for producing: Membrane proteins Secreted proteins

Lemo21(DE3)2 plasmid expression system Xbrane Bioscience Stockholm University

Protein Expression Protocol example: pET21 construct BL21(DE3) Lemo21(DE3) Transform, select on Amp plates Inoculate starter culture Inoculate expression culture Grow to mid-log: induce with 40-400 uM IPTG Continue growing 3-20 hours Harvest cells Transform, select on Amp, Cam plates Inoculate starter culture Inoculate expression culture, Add 0-2000 uM L-rhamnose Grow to mid-log: induce with 400 uM IPTG Continue growing 3-20 hours Harvest cells Important: IPTG level is not varied Only rhamnose is varied

Example of membrane protein expression optimization 100uM IPTG 0 100 500 1000 uM rhamnose 400 uM IPTG 0 100 500 1000 uM rhamnose 400 uM IPTG p8CBD-PhoA expression 22 hr Results Samuelson lab September 2008

NiCo21(DE3) -designed for the expression and purification of His-tagged proteins BL21(DE3) derivative: endogenous GlmS is mutated (6His to 6Ala) and 3 host metal binding proteins are tagged with chitin binding domain (CBD) Ni-NTA ↵  target      metal-chelate column chitin column target target  NiCo21(DE3)  Expression of His-tagged target protein Removal of CBD-tagged contaminants by chitin beads

NiCo21(DE3) outperforms BL21(DE3) for final protein purity BL21(DE3) NiCo21(DE3) M= ColorPlusprestained protein ladder L = Ni-NTA Load ft = Ni-NTA flow-through E = Ni-NTA Elution FTC = chitin column flow-through M L ft E L ft E FTC 175 ArnA-CBD 80  58 wt ArnA Glutamyl-tRNA synthetase(6His) 46  wt GlmS 30 SlyD-CBD 23 wt SlyD 17 7 81 85 97 % purity

+ cytoplasmic isomerase/ chaperone SHuffleTM a novel E. coli strain capable of correctly oxidizing proteins oxidizing periplasm oxidizing and reducing cytoplasm SHUFFLE wt+

Cys CH2 S S CH2 Cys Disulfide Bond Formation Cys CH2 SH Reduction + 2H+ + 2e- Oxidation SH acceptor CH2 O2 or enzyme catalyst e.g. DsbA Cys

disulfide bonds are important for protein folding and stability • found in secreted extracytoplasmic proteins: • e.g. antibodies, hormones, proteases, cytokines

trx/grx dsbC trx/grx dsbC SHuffle = Origami + cytoplasmic DsbC oxidizing cytoplasm periplasm

Available from NEB SHuffle Express SHuffle T7 Express SHuffle T7 Express lysY SHuffle T7 E. coli B E. coli K12

For licensing information regarding: the SHuffle strains, NiCo21(DE3) or Lemo21(DE3) Please contact the NEB business development office Email address: bus.dev@neb.com

Additional resources may be found at www.neb.com https://www.neb.com/tools-and-resources/selection-charts/competent-cell-product-comparison

Global Sales Review September 2008