Overview

NZCYM Broth is the highest-titre common broth for bacteriophage λ work and the global reference base for λ-derived molecular biology — library plating, screening, packaging extracts, cosmid propagation, and BAC handling. Originally formulated by Blattner, Williams, Blechl et al. in 1977 for the Charon-phage replacement vector series (Science 196: 161), the NZCYM design has three defining features that make it superior to LB and 2×YT for λ work: (i) NZ Amine, an enzymatic casein digest from Sheffield Bio-Science / Kerry with very low free-amino-acid asymmetry, (ii) casamino acids as a supplementary defined amino-acid pool, and (iii) built-in MgSO4 at 8.1 mM, well above the ~ 2 mM minimum required for stable λ tail-attachment to the LamB outer-membrane receptor, and within the 8–10 mM band that supports maximal adsorption rate without precipitation.

The GMExpression formulation is supplied as a pre-balanced dehydrated base (NZ Amine 10 g/L, casamino acids 1 g/L, yeast extract 5 g/L, NaCl 5 g/L, MgSO4·7H2O 2 g/L; total 23 g/L) ready for autoclave-and-use. Optional maltose stock (filter-sterilised 20 % w/v) provides the lamB-operon induction needed for high-efficiency library plating; optional top-agar (0.6 % w/v) and base-agar (1.5 % w/v) packs complete the λ plaque-assay supply chain. Typical liquid lysate titre on the standard λ host LE392: 1010–1011 PFU/mL — the highest of any common phage broth.

We also have

LB Broth (Miller) · LB Broth (Lennox) · 2×YT Broth (high-density host broth) · Bacteriophage Nutrient Broth (ΦX174 propagation grade) · TSB + 10 % Glycerol (host cryostock) · SM Buffer (phage diluent / storage) · BHI Broth (Gram-positive phage hosts)

Package Contents

Standard pack:

  • Mixture — pre-weighed dehydrated NZCYM base (NZ Amine 50 g, casamino acids 5 g, yeast extract 25 g, NaCl 25 g, MgSO4·7H2O 10 g; total 115 g for 5 L final volume). Sheffield Bio-Science / Kerry NZ Amine A locked supplier. Triple-foil-pouched; CofA traceable.

Optional stock:

  • Stock Mal (optional) — 20 % w/v D-maltose monohydrate, filter-sterilised at 0.22 µm, sterile-fill 25 mL amber vial; dosed at 10 mL/L for 0.2 % w/v final (= 5.5 mM); pre-induces lamB on the host before λ infection.

Alternative pack:

  • Top-agar pack (optional) — pre-weighed bacteriological agar (6 g per 1 L) for the 0.6 % w/v soft-agar overlay in λ plaque assays and library plating.
  • Base-agar pack (optional) — pre-weighed agar (15 g per 1 L) for plaque-assay base plates.

Customisation options on request: NZYM variant (omit casamino acids), NZY variant (omit casamino acids and Mg2+), animal-origin-free NZCYM (soybean substitute for NZ Amine), low-endotoxin NZCYM for vaccine-vector packaging, ampicillin-supplemented NZCYM for cosmid selection.

Composition — per 1 L equivalent unless stated otherwise

NZCYM Broth (Blattner et al. 1977 / Sambrook & Russell 2001 / BD Difco 244830; per 1 L)

ComponentConcentrationFunction
NZ Amine (Sheffield / Kerry enzymatic casein digest)10.0 gPrimary nitrogen and free amino-acid source with defined low amino-acid asymmetry; the "NZ" in NZCYM
Casamino acids (acid-hydrolysed casein)1.0 gSupplementary free amino acid pool; the "C" in NZCYM
Yeast extract5.0 gB-vitamins, purines, pyrimidines, NAD precursors; the "Y" in NZCYM
Sodium chloride (NaCl)5.0 gOsmotic balance (86 mM)
Magnesium sulfate heptahydrate (MgSO4·7H2O)2.0 g (= 8.1 mM Mg2+)The "M" in NZCYM — stabilises λ tail attachment to LamB; required cofactor for λ DNA replication

Total dry solids: 23 g/L. Pre-autoclaving pH: 7.0 ± 0.2 at 25 °C; typically requires < 0.2 mL of 5 M NaOH per litre to reach pH 7.0. Unlike LB-Mg, NZCYM does not phase-separate or precipitate on autoclaving because the MgSO4 is balanced against the casamino-acid load.

Optional supplements

SupplementFinal concentrationUse caseNotes
D-Maltose monohydrate (CAS 6363-53-7)0.2 % w/v (= 5.5 mM)λ library plating; λ high-titre lysateFilter-sterilise 20 % w/v stock; add 10 mL/L; pre-grow host to OD600 1.0 in NZCYM-maltose before infection — induces lamB
Additional MgSO4·7H2O+ 1–2 mM (top-up to 10 mM)Long lysate runs where Mg2+ is depleted by host metabolismAdd 1–2 mL of 1 M sterile filtrate per litre post-autoclave
Ampicillin / kanamycin50–100 µg/mLCosmid / BAC selectionStandard antibiotic selection; add post-autoclave
Agar (top agar)6–7 g/L (0.6–0.7 % w/v)λ plaque assay overlay; library platingAdd before autoclaving; equilibrate to 50 °C before mixing with phage and host
Agar (base agar)15 g/L (1.5 % w/v)λ plaque-assay base platesPour 20 mL per 90 mm plate

NZCYM variants

  • NZYM — omit casamino acids. NZ Amine + yeast extract + Mg2+. Slightly cheaper; ~ 20 % lower λ titre on fastidious hosts.
  • NZY — omit casamino acids and Mg2+. NZ Amine + yeast extract only. Used as a substrate-defined base where Mg2+ is dosed downstream.
  • NZCYM + 0.2 % maltose ("NZCYM-Mal") — the standard library-plating base; lamB-induced.

Culturomics and Media Navigator

Need help matching this medium to your λ-vector / cosmid / BAC workflow — or starting from a packaging-extract specification and finding the medium that fits? Use the GMExpression Culturomics and Media Navigator: a curated, cross-referenced tool that lets you (i) start from a medium and view supported λ vector classes and host strains, or (ii) start from a vector (Charon, EMBL3/4, λFIX, λZAP, cosmid pJB8, BAC pBeloBAC11) and view the panel of GMExpression media for propagation, plating, and packaging. The Navigator integrates NZCYM with the wider LB, 2×YT, Bacteriophage Nutrient Broth, BHI, SM Buffer, TSB–Glycerol, PPLO, Hayflick, and SP-4 catalogue.

Use and Applications

  • High-titre λ liquid lysate. Pre-grow LE392 (or another lamB+ host) in NZCYM + 0.2 % maltose to OD600 0.5; infect with λ at MOI 0.01; incubate 3–5 h at 37 °C until visible clearing; add 1 % chloroform, vortex, centrifuge, filter. Typical titre 1010–1011 PFU/mL.
  • λ genomic library plating and screening. NZCYM + 1.5 % agar plates + maltose-induced host + 50 µL library + 3 mL NZCYM + 0.6 % top agar; pour overlay; 8–18 h at 37 °C. Standard Charon, EMBL3/4, λFIX, λDASH, λZAP library protocol.
  • λ packaging-extract production. NZCYM as the growth medium for the lysogenic strains BHB2688 and BHB2690 producing the head- and tail-protein fractions of Gigapack-style packaging extracts; standard Stratagene / Promega / NEB packaging extract protocol.
  • Cosmid library propagation. NZCYM + ampicillin or kanamycin for routine growth of cosmid-containing hosts (pJB8, pHC79, SuperCos, cKM cosmids).
  • BAC propagation. NZCYM + chloramphenicol 12.5 µg/mL for pBeloBAC11-, pBAC108L-, pCC1BAC-derived BACs; supports single-copy maintenance with low recombination.
  • λ lysogen induction and excision. NZCYM is the standard broth for thermal induction of λcI857 lysogens (shift from 30 to 42 °C) and for mitomycin-C-induced lytic-cycle activation.
  • Cre/loxP subcloning of λ or cosmid inserts — the Cre recombinase (a P1 phage site-specific recombinase, not a λ recombinase) catalyses excision / integration between loxP sites in NZCYM-grown hosts; routine subcloning, vector retrofitting, and BAC end-clone rescue.

Compatible Microorganisms

Lambda host strains (primary use)

  • E. coli LE392 (hsdR514, supE44, supF58, lacY1, galK2, galT22, metB1, trpR55) — classic λ-vector plating host; reference NZCYM strain
  • E. coli Y1090 (r−, m−, supF, lacU169, hsdR, pMC9) — λgt11 expression-library screening host
  • E. coli MM294 (hsdR−, supE) — cosmid plating host
  • E. coli Q358, Q359 — Charon-vector plating
  • E. coli XL1-Blue MRF' (mcrA, mcrB, mcrCB, hsdSMR, mrr) — λZAP and λDASH plating
  • E. coli SURE, SURE-2 — recombination-suppressing λ-cloning hosts
  • E. coli BHB2688, BHB2690 — packaging-extract producer strains (cI857 lysogens)
  • E. coli P2392 — Spi-selection λ library plating

Cosmid and BAC hosts

  • E. coli ED8767, DH1, DH5α-MCR — cosmid propagation
  • E. coli DH10B, EPI300 — BAC and fosmid propagation; copy-control compatible
  • E. coli NS3145, NS3622 — recombineering hosts (galK, galETKM positive selection)

Not optimised for: ΦX174 (use LB Lennox + 5 mM Ca2+), filamentous M13 (use 2×YT — the Mg2+ in NZCYM is unnecessary), Gram-positive phages (use BHI), Φ6-class enveloped phages (use cyanobacterium-derived media), mycobacteriophages (use Middlebrook 7H9).

Preparation

1Weigh. Use the pre-weighed Mixture A: 23 g for 1 L. Tare a clean autoclavable Schott bottle of at least 1.5× final volume.
2Suspend & dissolve. Add Mixture A to 950 mL of distilled or deionised water (Type II reagent water, > 1 MΩ·cm). Stir for 5–8 min until fully dissolved; the MgSO4 dissolves with mild endothermic cooling.
3Adjust pH. Check pH with a calibrated meter; target 7.0 ± 0.2 at 25 °C. The base typically reads pH 6.8–6.9 before adjustment; titrate with 5 M NaOH (typically < 0.2 mL/L) to bring to pH 7.0.
4Bring to final volume. Make up to 1000 mL with distilled water.
5Dispense. Bulk flasks: leave caps one-quarter turn loose. For λ library plating, partition into 100–500 mL aliquots so the same broth base is used for top agar and bottom agar on each plate.
6Autoclave. 121 °C × 15 min for ≤ 500 mL; 121 °C × 20 min for 1 L bottles. Slow cooling.
7Cool to < 50 °C before adding post-autoclave supplements (maltose, antibiotics).
8Add maltose for λ library plating. Aseptically add 10 mL of 20 % w/v sterile maltose per litre (= 0.2 % final). Pre-grow the host in this NZCYM-maltose to OD600 1.0 before infection — this is the lamB-induction step that gives the 10–100× titre boost.
9Plaque assay overlay (DAL). Mix 50 µL λ library + 200 µL host (OD600 1.0 in NZCYM-Mal) in 3 mL NZCYM top agar (0.6 %, equilibrated to 50 °C); pour over NZCYM base agar (1.5 %); incubate 37 °C 8–18 h.
10Storage. Sealed glass bottles at 2–8 °C, light-protected. NZCYM is unusually stable on storage because the built-in MgSO4 does not precipitate without phosphate.

Critical control points

  • Maltose pre-induction is non-negotiable for library work. The lamB-encoded outer-membrane LamB porin is the λ J-protein adsorption receptor. Without maltose induction (or constitutive lamB) the host adsorption rate is 10× slower and the plaque count drops proportionally. Pre-grow the host in NZCYM + 0.2 % maltose for ≥ 2 generations before infection; harvest at OD600 1.0 (not 0.5; library plating uses denser hosts than liquid lysates).
  • NZ Amine supplier lock. NZ Amine is manufactured by Sheffield Bio-Science (subsequently Kerry). Generic "casein peptone" substitutes are not equivalent — the free amino-acid profile differs, and side-by-side bench comparisons consistently show lower λ titre and reduced library complexity. Lock the supplier on the CofA.
  • Top-agar equilibration temperature. Soft (0.6 %) NZCYM agar must be held at 50 °C ± 2 in a water bath. Above 55 °C the host suffers heat-shock loss; below 48 °C the agar starts to set during mixing and gives a granular overlay. Use an immersion thermometer rather than the bath setpoint.
  • Same base for top and bottom agar. Use NZCYM for both layers in the plaque assay. Mixing NZCYM bottom with LB top (or vice versa) causes ion-strength shifts during overlay equilibration that distort plaque morphology and reduce visible plaque count.

Cautions

NZ Amine supplier substitution. Generic "casein peptone" or "NZ Amine Type S/A" lots from non-Sheffield/Kerry sources are not equivalent. The defining feature of NZ Amine is its very low free-amino-acid asymmetry and consistent free-tryptophan content — both of which directly affect λ gene-expression rate during library plating and packaging-extract preparation. Specify Sheffield/Kerry NZ Amine A on every CofA; do not accept generic substitutes for regulated workflows.
Maltose stability. Sterile 20 % maltose stock degrades by ~ 5 % per month at 2–8 °C via slow disproportionation to glucose + reducing sugars. Aliquot in 25 mL single-use vials at −20 °C for long-term storage; once thawed, use within 2 weeks. Do not autoclave maltose with the broth — caramelisation produces inhibitory furans that reduce λ titre.
Mg2+ depletion during long lysate runs. Host metabolism consumes free Mg2+ into rRNA-bound and ribosome-bound pools; in long (> 6 h) lysate runs the free Mg2+ can drop below the 2 mM threshold required for λ tail attachment, prematurely capping the burst. For runs > 5 h, supplement with 1–2 mL of 1 M sterile MgSO4 per litre mid-run to top up to 10 mM.
Packaging-extract producer strains. BHB2688 (head-protein producer) and BHB2690 (tail-protein producer) carry λcI857 temperature-inducible lysogens. Maintain at 30 °C (no induction) on NZCYM + Amp; induce by shift to 42 °C for the packaging-extract protocol. Accidental warming above 32 °C during routine handling causes partial induction and loss of producer-strain stability.
Cosmid / BAC recombination. Long-incubation NZCYM cultures of cosmid- or BAC-bearing hosts can lose insert via RecA-dependent recombination on repeated subculture. Use Rec hosts (DH10B, SURE, NS3622) for stable BAC propagation; subculture as few times as possible from a frozen stock; verify insert by restriction mapping every 3 subcultures.

Storage and Expiry · Safety

  • Dehydrated powder (Mixture A): store sealed at 15–25 °C in original packaging away from direct sunlight. Shelf life 24 months from manufacture (slightly shorter than LB due to MgSO4 hygroscopicity).
  • Sterilised broth (unsupplemented): 2–8 °C in sealed glass, 6 months; no Mg-precipitation on long storage because phosphate is absent.
  • Sterilised broth + maltose: 2–8 °C, 2 weeks.
  • Sterilised broth + antibiotic: antibiotic-dependent; ampicillin 1 week, kanamycin 4 weeks, chloramphenicol 4 weeks.
  • Maltose 20 % stock: −20 °C aliquots, 12 months; 2–8 °C, 2 weeks.
  • Poured NZCYM agar plates: 2–8 °C in sealed bags, 4 weeks; bring to room temperature before plating to avoid condensation.

Safety notes. NZCYM is a non-hazardous routine bacterial broth. The principal biosafety concerns are (i) host strain BSL (most λ-host strains are BSL-1), (ii) chloroform vapour during lysate processing (handle in a fume hood; never autoclave chloroform), and (iii) λ packaging extracts (the lytic packaging strains are BSL-1 but should be handled in a Class II BSC to prevent cross-contamination with other λ libraries). SDS available on request.

References

  1. Blattner, F. R., Williams, B. G., Blechl, A. E., Denniston-Thompson, K., Faber, H. E., Furlong, L.-A., Grunwald, D. J., Kiefer, D. O., Moore, D. D., Schumm, J. W., Sheldon, E. L., Smithies, O. (1977). Charon phages: safer derivatives of bacteriophage lambda for DNA cloning. Science 196: 161–169. [Original NZCYM reference]
  2. Sambrook, J. & Russell, D. W. (2001). Molecular Cloning: A Laboratory Manual, 3rd ed., CSH Press. Chapter 2 (Bacteriophage λ).
  3. Frischauf, A. M., Lehrach, H., Poustka, A., Murray, N. (1983). Lambda replacement vectors carrying polylinker sequences. Journal of Molecular Biology 170: 827–842.
  4. Hohn, B. & Murray, K. (1977). Packaging recombinant DNA molecules into bacteriophage particles in vitro. Proceedings of the National Academy of Sciences USA 74: 3259–3263. [BHB2688/BHB2690 strain origin]
  5. Karn, J., Brenner, S., Barnett, L., Cesareni, G. (1980). Novel bacteriophage λ cloning vector. Proceedings of the National Academy of Sciences USA 77: 5172–5176.
  6. Kim, U. J., Birren, B. W., Slepak, T., Mancino, V., Boysen, C., Kang, H. L., Simon, M. I., Shizuya, H. (1996). Construction and characterization of a human bacterial artificial chromosome library. Genomics 34: 213–218.
  7. BD Difco & BBL Manual, 12th ed., NZCYM Broth monograph (BD 244830); Sigma N4019 specification.
  8. Murray, N. E. (2000). Lambda II in molecular biology — a personal view. In Hendrix, R. W. & Roberts, J. W. (eds), Lambda II, CSH Press.

Frequently Asked Questions

Q1. Why does NZCYM give a higher λ titre than 2×YT + Mg2+?
Two reasons. First, NZ Amine has a more balanced free amino-acid profile than tryptone, which gives a smoother growth curve and a more reproducible burst-size window. Second, casamino acids provide a defined supplementary pool of free amino acids that the host can immediately drive into λ capsid-protein synthesis during the lytic phase, increasing burst size by 20–40 % vs 2×YT. The built-in 8.1 mM Mg2+ is also pre-balanced against the casamino-acid load to avoid the Mg-citrate / Mg-acetate sequestration that occurs in some 2×YT-Mg formulations.
Q2. What is the difference between NZCYM, NZYM, and NZY?
NZCYM = NZ Amine + Casamino acids + Yeast extract + Magnesium (full formulation; reference for library work and high-titre lysate). NZYM = NZ Amine + Yeast extract + Magnesium (omits casamino acids; ~ 20 % lower λ titre on fastidious hosts). NZY = NZ Amine + Yeast extract (omits casamino acids and Mg2+; used as a substrate-defined base where Mg2+ is dosed downstream). Default to NZCYM unless cost optimisation or upstream Mg2+ control dictates otherwise.
Q3. Can I substitute generic casein peptone for NZ Amine?
Not for regulated workflows. The defining feature of NZ Amine (Sheffield Bio-Science / Kerry NZ Amine A) is its very low free-amino-acid asymmetry and consistent free-tryptophan content, both of which directly affect λ lytic-cycle gene expression rate. Generic casein peptone substitutes give measurably lower λ titre and reduced library complexity in side-by-side comparisons; the precise magnitude varies with the specific substitute peptone, with reductions in the order of tens of percent commonly reported. For routine non-regulated work the substitution may be acceptable with a documented titre cost; for λ library plating, packaging-extract production, or any GMP/cGMP workflow lock the NZ Amine supplier.
Q4. Why does library plating use OD600 1.0 host instead of OD600 0.5?
Library plating density is set by the host-cell concentration in the top agar, which determines the lawn density of the overlay. Plaque morphology is best when the host concentration is ~ 5–10 × 108 CFU/mL in the top agar, corresponding to OD600 ~ 1.0 from a saturated NZCYM-maltose pre-culture. OD600 0.5 (mid-log) gives a thinner lawn that visualises plaques less crisply and increases the risk of plaque coalescence at high library titres. Liquid lysate work, in contrast, harvests at mid-log for maximum burst-size; the two density rules apply to different steps.
Q5. Why is there no phosphate buffer in NZCYM?
Phosphate would precipitate Mg2+ as insoluble Mg-phosphate, removing the 8 mM Mg2+ that defines NZCYM's λ performance. The pH of NZCYM is stabilised by the inherent buffering of the peptide / amino-acid pool and by the yeast-extract phosphate (~ 3–5 mM, sub-precipitation threshold against 8 mM Mg2+). For very long lysate runs where pH drift is a concern, use Tris-HCl 10 mM as a top-up buffer; never substitute phosphate.
Q6. Can I use NZCYM for BAC propagation, or only for cosmid?
Yes, NZCYM is fully compatible with single-copy BAC propagation. Standard BAC hosts (DH10B, EPI300) grow well in NZCYM + chloramphenicol 12.5 µg/mL; the higher amino-acid content vs LB supports the very low growth-rate demands of single-copy BACs without selecting for high-copy recombinants. For copy-control BAC vectors (pCC1BAC), use NZCYM + chloramphenicol routine maintenance + L-arabinose 0.01 % induction at harvest. Sub-culture as few times as possible to limit RecA-mediated insert loss.
Q7. Why does my λ plaque assay show "halo plaques"?
Halo plaques (small dense centre with translucent halo) usually indicate (i) excess Mg2+ driving over-efficient adsorption that overwhelms the host density, or (ii) host strain expressing inhibitory factors. Check the actual Mg2+ concentration (8–10 mM is optimal; > 15 mM gives halos); verify the host is LamB+ (no malB mutation); confirm the host was maltose-induced before plating. If halos persist, dilute the library 10× further and re-plate — very high plaque densities also look halo-like due to plaque coalescence.
Q8. Is NZCYM the right broth for λ helper-phage rescue of vectors like λ-ZAP?
Yes — λZAP is rescued in NZCYM + maltose using XL1-Blue MRF' or a similar host with the M13K07 / ExAssist helper phage. The NZCYM Mg2+ supports both the λ replication phase and the helper-phage rescue phase; the maltose induces lamB for any residual λ activity. Follow the standard Stratagene / Agilent λZAP / ExAssist protocol; NZCYM is the medium-of-record in the kit documentation.