J. AOAC Int. 81, 51-56 (1998). TLC of 6 sulfonamides (sulfadimidine, sulfadoxine, sulfadiazine, sulfadimethoxine, sulfathiazole, sulfamerazine) on silica gel with concentration zone with mixtures of NH3 in methanol and dichloromethane and a 3-step TLC method acc. to L.S.G. van Poucke et al., J. Chromatogr. Sci. 29, 423-427 (1991). Detection after drying by dipping in a 0.01% fluorescamine in acetone solution and observation under UV 366 nm. Semiquantitative determination by visual comparison of the spots against spiked samples.

J. Planar Chromatogr. 14, 350-354 (2001). TLC of troleandomycin, tylosin, rifamycin B, vancomycin, erythromycin, and rifampicin on polyamide 11 plates with five binary solvent mixtures methanol - water, ethanol - water, propanol - water, acetonitrile - water, and tetrahydrofuran - water. Detection by spraying with anisaldehyde - methanol - acetic acid - orthophosphoric acid - sulfuric acid 1:100:10:10:5 and heating at 110°C for 10 min.

J. Planar Chromatogr. 18, 423-426 (2005). HPTLC of antibiotics (sulfadimidine, sulfadiazine, sulfaguanidine, trimethoprim) on silica gel without chamber saturation in a twin-trough chamber with chloroform - methanol 89:11. Quantification by videodensitometry at 254 nm. Limit of detection was 0.05 µg per spot for sulfadimidine, sulfadiazine, and sulfaguanidine, and 0.1 µg per spot for trimethoprim.

Food Chem. 177, 354-360 (2015). HPTLC of ochratoxin A in rice bran, wheat bran and wheat flour on silica gel with n-hexane - ethyl acetate - acetic acid 36:8:3. Quantitation by absorbance measurement at UV 366 nm. Linearity was between 50 and 300 ng/zone. The LOD and LOQ for ochratoxin A was 10 and 30 ng/zone, respectively. Recovery was in the range of 86-113 %.

Prepacked-column extraction and quantitative HPTLC-determination of the aflatoxins B1, B2, G1 and G2 in fungal suspensions.) Fresenius Z. Anal. Chem. 319, 527-532 (1984). Quantitative determination of aflatoxins by HPTLC after prepacked column extraction. HPTLC on silica with chloroform - acetone 9:1 and post-chromatographic treatment with paraffin - hexane 1:2. In-situ fluorescence scanning at 344/430 nm.

Anal. Chim. Acta 170, 149-152 (1985). Two-dimensional TLC of aflatoxin M1 on silica with ether - methanol water 95:4:1 in the 1st direction, chloroform - acetone 7:3 in the 2nd direction. Quantitation by fluorescence densitometry. Detection limit 0.005 ng/g for milk and 0.05 ng/g for milk powder.

J.A.O.A.C. 68, 1126-1128 (1985). TLC of deoxynivalenol (vomitoxin) on silica with ethyl acetate and chloroform - acetone - isopropanol 8:1:1. Detection by dipping in aluminium chloride solution and heating on a (preheated) hot plate for 5 min. and observation under UV 366 nm.

J. Agric. Food Chem. 35, 354-358 (1987). TLC identification of (3H) T-2 and metabolites on silica with e.g. ethyl acetate - toluene 3:1 or diethylether - acetone 1:1. Visualization by first spraying with Scinti Pre. (Fisher) and then exposing the plates to x-ray film. Quantification by scraping the appropriate gel regions and subjecting them to LSC analysis.