Lipids 17, 515-518 (1982). TLC of acidic lipids on silica after column chromatography with chloroform - methanol - 0.25 % KCl 60:35:8. Detection with bromothymol blue. Zones scraped off. Elution of the indicator with chloroform - methanol 8:2 and of cholesterol glucuronide and ganglioside with chloroform - methanol 5:5.

Anal. Letters 18, 609-616 (1985). TLC of phospholipids and neutral lipids of E. coli on silica with a) chloroform - methanol - 0.25 % NaCl water solution - iso-propanol - triethylamine 40:10:6:25:18, b) chloroform - methanol - iso-propanol - ethyl acetate - triathylamine 30:10:25:7:35, c) hexane -ether - formic acid 80:20:2. Detection by spraying with conc. sulfuric acid - ethanol - water 34:33:33 and heating at 140 °C. Densitometry.

VIII. Separation of l-o-acetylethylene glycol-2-(2-trimethyl-ammonium-ethyl) and -(2-aminoethyl) phosphonates from their phosphoryl analogues and other phosphonolipids. J. Chromatogr. 351, 376-378 (1986). TLC of l-o-acetylethylene glycol-2-(2-trimethyl-ammoniumethyl) and-(2-aminoethyl) phosphonates on silica with a) chloroform - methanol - water 65:25:4, b) methanol - water 2:1. Detection by exposure to iodine vapor, or UV irradiation, or spraying with molybdenum blue.

H. TRAITLER, A. STUDER, R.E. KAISER (eds): Instrumental HPTLC, Institute for Chromatography, Bad Dürkheim, FRG (1987), 101-109. TLC of phospholipids and glycolipids on silica with chloroform - methanol - triethylamine - water 30:35:34:8 and chloroform - methanol - 0.25% calcium chloride 60:35:8, resp. Detection by dipping in TNS reagent and photographing on film negatives. Measurement by laser scanning in transmittance mode. Detection limit, 25 ng.

J. Chromatogr. 409, 291-7 (1987). TLC on 5% silver nitrate-impregnated silica developed to 3 cm above the origin with chloroform - methanol - water 70:30:4, and to 16 cm with chloroform - methanol - water 90:10:1. Analysis by enzymatic radioacitve phosphorylation.

J. Chromatogr. 426, 188-193 (1988). TLC of 6 neutral glycosphingolipids on silica with 4 solvent systems composed of isopropanol, 15M NH3, methyl acetate and water. Detection by spraying with 50% sulfuric acid and heating at 110°C.

Anal. Biochem. 173, 10-17 (1988). HPTLC on silica with acetone - 5N NH3 50:0.9. Detection by autoradiography. Liquid scintillation, spectrometry after scraping. Fixation of the silica gel and treatment with neuraminidase from Vibrio cholerea in the absence of detergent and incubation of the plates with antibodies. Visualization of bound first antbodies by using alkaline phosphatase conjugated second antibodies. Detection limit, 30 ng.

J. Liquid Chromatogr. 12, 3151-3161 (1989). TLC of sterols and other lipids on silica with isopropyl ether – acetic acid 96:4, followed by hexane – ether – acetic acid 90:10:1. Detection of lipids by spraying with 5% ethanolic phosphomolybdic acid and heating for 5-10 min at 100-120°C. Semiquantification by comparison of the zone sizes and intensities of standards and samples. Quantification of cholesterol by densitometry after development with chloroform – ethyl acetate 96:4, and dipping in cupric acetate – phosphoric acid reagent and heating at 100°C. Quantification of triacylglycerols and free fatty acids by densitometry after development with hexane – ether – acetic acid 80:20:1, followed by spraying with cupric acetate – phosphoric acid reagent. Also GC.