Planta Medica 84(12-13), 902-912 (2018). A dichloromethane extract of Athrixia phyllicoides aerial parts (Asteraceae) was eluted on a silica gel column with different mixtures of ethyl acetate and hexane or methanol. This fractionation was monitored on TLC silica gel layers, using the combinations of the same solvents as mobile phases. Detection by derivatization with Natural Product Reagent and PEG, and visualization at UV 254 nm. This allowed the grouping of the fractions into 13 profiles and the isolation of three hydroxy-methoxyflavones and a coumarate.

J. Planar Chromatogr. 33, 281-291 (2020). HPTLC of Weikangling capsules (a Chinese patent medicine for treating chronic gastritis, containing Paeoniae Radix Alba, Glycyrrhizae Radix et Rhizoma, Bletillae Rhizoma, Notoginseng Radix et Rhizoma, Poria, Corydalis Rhizoma, Sepiae Endoconcha, and Belladonnae Extractum) on silica gel with chloroform - methanol - water 14:5:1. Detection by spraying with 10 % sulfuric acid in alcohol, followed by heating at 105 ºC for 5 min. Qualitative analysis at UV 366 nm.

Phcog. Mag. 15, 440-448 (2019). HPTLC fingerprint of Psidium guajava on silica gel with toluene - ethyl acetate - formic acid 6:3:1. Qualitative determination under UV light at 254 and 450 nm. The hR_F values of common metabolites were 3, 18 and 42 in both aqueous and n‑butanol fractions.

Phytochem. Anal. 31, 57-67 (2019). HPTLC profiling of the leaves of Fraxinus excelsior on silica gel with ethyl acetate - water - formic acid 8:1:1. Qualitative identification under UV light at 254 and 366 nm. The hR_F value of chlorogenic acid was 90.

Planta Medica 84(9/10), 584-593 (2018). A review with 120 references on DESI technique coupled with MS for natural products. Paragraph on sample preparation (9 references) compares analyte desorption surfaces: either directly from the biological sample, or indirectly from surfaces on which the sample had been imprinted. Direct desorption can be performed only from samples with hard, smooth and regular surfaces, or from cryosections, which are usual for animal tissues. For plants, indirect analysis is preferable because of their wax-rich, hydrophobic, absorbent and/or irregular surfaces. Imprinting of plant organs and tissues can be performed either on glass (however with a very rapid ablation of the analytes from its surface), or on sorbent material, like TLC silica gel or porous polytetrafluoroethylene (PTFE). While PTFE layers are reported as more expensive and better in terms of reproducibility and quantitative analysis, both TLC and PTFE layers have similar performance for analyte retention until desorption.

Planta Medica 84(9/10), 710-715 (2018). The fractionation of an n-butanol extract of Cistanche phelypaea (Orobanchaceae) aerial parts through cyclodextran column chromatography with methanol was monitored on TLC silica gel with chloroform – methanol – water 70:30:3, detection by spraying with cerium sulfate reagent. In the 11 major fractions obtained, 4 new phenylethanoid glycosides were further identified, as well as brandioside (a phenylpropanoid glycoside), and heterosides of apigenin (flavonoid) and of pinoresinol (lignan).

Planta Medica 84(9/10), 716-720 (2018). The fractionations of n-hexane and chloroform extracts of Guarea guidonia aerial parts (Meliaceae) through silica gel column chromatography was monitored on TLC silica gel with cerium sulfate / sulfuric acid as derivatization reagent. In the fractions obtained, 3 new tirucallane-type triterpenoids (guareolide, guareoic acids A and B) were further identified, as well as other terpenoids (flindissone, acetyldihydronomilin, picroquassin E, boscartol C, and acneorubins A, B, and X).

Planta Medica 84(9/10), 729-735 (2018). The chloroform fraction of a methanolic extract of Euphorbia taurinensis whole plant (Euphorbiaceae) was submitted to a multi-step fractionation through column chromatography. Monitoring by TLC on silica gel (mobile phases see below) followed by derivatization with concentrated sulfuric acid and heating at 105°C. The fractions obtained were purified by repeated cycles of preparative TLC alone or alternating with preparative HPLC, leading to the isolation of segetane, ingenane, and jatrophane diterpenes. Depending on the subfractions, preparative TLC silica gel and reverse-phase C18 layers were used, with cyclohexane – ethyl acetate – ethanol 25:15:1 for normal phase, and with mixtures of acetonitrile (or methanol) and water for RP.