Antibiotics

Antibiotic sensitivity varies substantially among species of labyrinthulomycetes.

Inhibitory concentrations of various antibiotics for diverse labyrinthulomycetes. ns indicates ‘not sensitive’. Tet=tetracycline, Dox=doxycycline, Nour=nourseothricin, Hyg=hygromycin B, G418=geneticin, Bek=bekanamycin, Kas=kasugamycin, Blast=blasticidin, Zeo=zeocin. Also screened and uniformly not inhibitory: penicillin, ampicillin, kanamycin, streptomycin, spectinomycin, carbenicillin, neomycin, puromycin. * indicates data from Sakaguchi et al. 2012.

Tet Dox Nour Hyg G418 Bek Kas Blast Zeo
Oblongichytrium sp.#
SEK600 250 2000 100 200
SEK600 400 2000 50 200 80
SEK707 400 2000 100 200 80
SEK708 50 ns 50 20 80
SEK711 50 2000 100 20 80
Aurantiochytrium limacinum
SR21# 250 2000 100 200 80
ATCC MYA-1381$ 100 100 100 200 500 ns 50 15
mh0186* ns 2000 2000 100 1000
Schizochytrium aggregatum
ATCC 28209$ 100 100 100 800 500 50
204-06 m* 2000 2000 ns ns
Thraustochytrium aureum
ATCC 34304* ns 2000 2000 100 ns
Parietichytrium
TA04Bb* 2000 2000 800 ns
Labyrinthula
KIE13% ns ns 50 ns
Aplanochytrium
PBS06$ 100 100
PBS07$ 100 100

This data was generated by Collier, Rest, et al. as part of a grant from the Gordon and Betty Moore Foundation.

#Honda et al. data: Strains were pre-cultured in 25ml of dGPY medium or Sea Act I medium in a 125 ml Erlenmeyer flask at 25C for 5 days. Growth assays were performed in 24 well plates (lumox multiwell plate/Sarstedt). Each well contained 1ml of dGPY and an appropriate concentration of an antibiotic. 10μl of pre‐cultured cells were transferred into each well and the plates were incubated at 25C. Optical density was measured on a plate reader (PerkinElmer ARVO MX 1420) at 610nm and at 25 points in each well 0h, 24h, 48h, 72, and 7days after inoculation. 

$Collier, Rest et al. data: Strains were pre-cultured in 25ml of full-strength 790 medium (Schizochytrium and Aurantiochytrium) or 10% 790 medium (Aplanochytriumin a 125 ml Erlenmeyer flask at 25C for 5 days. Growth assays were performed in 96 well plates. Each well contained 200 ul of growth medium and an appropriate concentration of an antibiotic. 10μl of pre‐cultured cells were transferred into each well and the plates were sealed and incubated at 25C, with shaking at 3,000 rpm for Schizochytrium and Aurantiochytrium. Optical density was measured on a plate reader (Tecan Inifinite F500) at 610nm and at 25 points in each well 0h, 24h, 48h, 72, and 7days after inoculation. 

%Reusch, Brakel et al. data: Labyrinthula strains were cultivated on serum seawater medium (1L miliQ water, 12g agar agar, 1g glucose, 0.1 g yeast extract, 0.1 g peptone, 10 ml horse serum and 25 ml penicillin-streptomycin, 25 g Instant Ocean) at 22°C in dark. Labyrinthula growth assays were performed in 6-well plates. In the middle of each well an agar disc from the growing front of a Labyrinthula culture growing on agar was placed upside down. Then the wells were filled by 2 ml of serum seawater medium including the respective antibiotic (method modified from Martin et al. 2009). The chambers were incubated at 22°C or 25°C in dark. After 24, 48 and 96 hours , cultures were inspected under a microscope with 60x magnification. The whole area of the well was inspected, and the area of highest cell concentration was photographed and cell density was categorized according to the following categories: (0) full coverage of bottom by cells, (1) cells in aggregates visible, (2) singular cells visible, (3) total absence.

 

Examples of microtiter plate growth curves showing zeocin sensitivity of Aurantiochytrium limacinum and resistance of Schizochytrium aggregatum and Thraustochytrium aureum