Strain modifications for Medium 381

Adjust pH of final medium to 6.0.

Add 100g NaCl (10%) for 1000 ml medium.

Add to medium Na-sesquicarbonate solution (1 mL in 10 mL) to achieve pH 9.5 plus CaCl₂. Na-sesquicarbonate solution: NaHCO₃ 4.2 g, Na₂CO₃ anh. 5.3 g, dist. water 100 mL

Agar plates with 1% hexadecane. Alternatively, place a drop of hexadecane on the lid of the petridish; Use 3 ml medium 1 or medium 381 for rehydration of freeze dried culture.

If used as phage host, growth at 32°C recommended

Medium for chitin decomposition see reference (9297).

Or any conventional minimal medium supplemented with 0.2% glucose and thiamine

Plus 0,35% Tween 80

Plus 10 mg/L MnSO₄

Plus 100 mM boric acid

Plus 2% NaCl

Plus 25 mg/l Cm

Plus 3% NaCl

Plus 3% NaCl (final concentration)

Plus ampicillin 100 mg/ml

Plus Kanamycin 50 mg/ml

Plus 0.2% glucose

plus 10% NaCl

plus 20g/l NaCl

plus 3% NaCl (final concentration)

Plus 50 mg/L Nalidixic acid

Rehydrate and grow cells from the ampoule in liquid medium. Subsequent subculturing may be carried out in liquid medium or on agar plates

Rehydrate and grow lyophilized cells from the ampoule in 5 ml liquid broth 1. Subsequent subculturing may be carried out in liquid medium or on agar plates

Rehydrate and grow lyophilized cells from the ampoule in 5 ml liquid broth 381. Subsequent subculturing may be carried out in liquid medium or on agar plates

Rehydrate and grow lyophilized cells in liquid broth 381. Subsequent subculturing may be carried out in liquid medium or on agar plates

Resuspend and grow freeze-dried cells from ampoules in liquid medium first. Subsequently, cultivation may be carried out in liquid medium and on agar plates.

Solified with 15 g/l agar

With kanamycin for selection

With only 5g/L NaCl and supplemented with 50 µg/mL 5-aminolevulinic acid (ALA)

+ 2% NaCl