Cumulative CAMAG Bibliography Service CCBS

Our CCBS database includes more than 11,000 abstracts of publications. Perform your own detailed search of TLC/HPTLC literature and find relevant information.

The Cumulative CAMAG Bibliography Service CCBS contains all abstracts of CBS issues beginning with CBS 51. The database is updated after the publication of every other CBS edition. Currently the Cumulative CAMAG Bibliography Service includes more than 11'000 abstracts of publications between 1983 and today. With the online version you can perform your own detailed TLC/HPTLC literature search:

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      130 141
      Two-dimensional high-performance thin-layer chromatography for the characterization of milk peptide properties and a prediction of the retention behavior – a proof-of-principle study
      M. TREBLIN, T. VON OESEN, L.-C. CLASS, G. KUHNEN, I. CLAWIN-RÄDECKER, D. MARTIN, J. FRITSCHE, S. ROHN* (*Department of Food Chemistry and Analysis, Institute of Food Technology and Food Chemistry, Technical University of Berlin, Berlin, Germany; rohn@tu-berlin.de)

      J Chromatogr A 1653, 462442 (2021). Samples were peptides obtained through tryptic hydrolysis of the 5 most abundant milk proteins: α-lactalbumin (α-LA), β-lactoglobulin (β-LG), α-, β- and κ-casein (CA). As standards, synthetic whey and pea (Pisum sativum, Fabaceae) peptides (selected based on the in silico tryptic digest of α-LA, β-LG, legumin A, and vicilin with one or zero miscleavages) were only used in the last assay for prediction of the RF values of peptides with known amino-acid (AA) sequences. Two-dimensional HPTLC on silica gel (pre-washed with methanol and activated 10 min at 100°), first with basic mobile phase sec-butanol – pyridine – ammonia – water 39:34:10:26, and (after 12h drying) in the orthogonal direction with acidic mobile phase sec-butanol – pyridine – acetic acid – water 11:8:2:5. Derivatization for peptides and proteins by immersion into fluorescamine (0.05 % in acetone); visualization under UV 254 nm and 365 nm. Computer-assisted determination of the x- and y-coordinates of the derivatized zones. Repeatability (n=8) of the 2D-HPTLC was statistically tested with the Kolmogorov-Smirnov test for normal distribution and with Dixon’s Q test for outliers. Relative standard deviation (RSD) for the RF values was 12.9 % for the first dimension (y-coordinates) and 16.5 % for the second dimension (x-coordinates). According to their higher intensity and sharpness, 15 – 20 detected zones from each protein hydrolyzate were selected, manually scraped from the derivatized layer, dissolved in formic acid solution (0.1 % in acetonitrile – water 3:2), mixed with an equal volume of matrix (dihydroxybenzoic acid 2 % in acetonitrile – water 3:7), crystallized on air on a ground steel target, before being desorbed by the laser beam of the MALDI-TOF-MS/MS (matrix-assisted laser desorption/ionization time-of-flight tandem mass spectrometry). Direct hyphenation of HPTLC to MS was not performed, to avoid zone diffusion during plate coating with the matrix and to circumvent the stronger binding of polar peptides on the layer.  The MS spectra were acquired in positive reflector mode in m/z range 340 – 4000 (10 – 2500 for fragments), using an external peptide as calibration standard. Identification of 51 from the 85 selected peptides according to AA sequences was performed, using software programs allowing m/z calculation of protein fragments and estimation of cleavage sites. Correlation of the retention behaviour of the peptides with their properties (molecular weight MW, isoelectric point IEP, charges, polarity) was tested with Student’s two-sided t-test after calculation of Pearson’s correlation coefficients. The correlation was significant with IEP, percentages of anionic AA and of non-polar AA; but not with the following properties: MW, percentages of cationic AA and of uncharged polar AA. Finally, based on the correlation results, regression formulas were found to calculate the x- and y-coordinates of any known peptide from the percentage of non-polar AA (or vice-versa). The prediction power of these formulas was verified by repeating the complete 2D-HPTLC-MS experiment with the standard peptides of whey and of peas, and measuring the absolute and relative deviations between the actual x- and y-coordinates and the predicted values. The absolute deviations were higher in the lower RF zones. The average, relative RF value deviations (range 22.1 – 25.7 %) were not different between whey and pea peptides.

      Classification: 2c, 2d, 4e, 18b, 19, 32e
      130 089
      Advances in analytical techniques coupled to in vitro bioassays in the search for new peptides with functional activity in effect-directed analysis
      Luz GUERRA*, J. PAVON, A. VALLEJOS, D. JORQUERA (*Department of Food Science and Technology, Faculty of Pharmacy, University of Concepcion, Chile, lguerra@udec.cl)

      Food Chem. 133784 (2022). Review of enzymatic protein hydrolysis, including standard and conventional techniques and their applications and insights into new strategies of detection and characterization of bioactive peptides. The paper described HPTLC methods coupled with bioassays in effect-directed analysis (EDA) to detect the bioactivities of peptides.

      Keywords: HPTLC review
      Classification: 18b
      130 029
      Efficient isolation of mycosporine-like amino acids from marine red algae by fast centrifugal partition chromatography
      M. ZWERGER, S. SCHWAIGER, M. GANZERA* (*Department of Pharmacognosy, Institute of Pharmacy, University of Innsbruck, Innsbruck, Austria; markus.ganzera@uibk.ac.at)

      Marine Drugs 20(2), 106 (2022). TLC was used to monitor the fractionation of hydro-methanolic extracts of Rhodophytes: Gracilaria gracilis (Gracilariaceae) (A), Porphyra sp. (Bangiaceae) (B), Spongoclonium pastorale (Ceramiaceae / Wrangeliaceae) (C); and to assess the purity of two isolated mycosporine-like amino acids: porphyra-334 and shinorine.  TLC on silica gel with n-butanol - acetic acid - water 3:1:1. Derivatization by spraying ninhydrin reagent for the detection of peptides and amino-acids; or by spraying anisaldehyde - sulfuric acid for most phytochemicals; in both cases, followed by 5 min heating at 100 °C. Visualization under white light and at 366 nm. Porphyra-334 (hRF 28) was isolated pure from (B) and (C). Shinorine (hRF 25), isolated from (A) and (B), contained a coeluting sugar (hRF 48), which was absent after further purification on solid phase extraction, and, only when isolated from (B), a coeluting peptide or amino-acid (hRF 35), which was absent after further purification on cyclodextrane column chromatography.

      Classification: 4d, 18a, 32e
      129 070
      Effect-directed screening of Bacillus lipopeptide extracts via hyphenated high-performance thin-layer chromatography
      M. JAMSHIDI-AIDJI, I. DIMKIC, P. RISTIVOJEVIC, S. STANKOVIC, Gertrud E. MORLOCK* (*Institute of Nutritional Science, and Interdisciplinary Research Centre for Biosystems, Land Use and Nutrition, Justus Liebig University Giessen, Giessen, Germany; gertrud.morlock@uni-giessen.de)

      J Chromatogr A, 1605, 460366 (2019). Samples were standards and complex mixtures of non-ribosomally synthesized cyclic lipopeptides (CLPs) from Bacillus strains (Bacillaceae) found in soil or in manure: B. amyloliquefaciens (SS-12.6, SS-13.1, SS-27.2, SS-38.4) and B. pumilus (SS-10.7). Two extraction methods were compared: ethyl acetate extraction (Ex1), and the acidic precipitation followed by methanol extraction (Ex2). HPTLC on silica gel with chloroform – methanol – water 65:25:4. Detection under white light, UV 254 nm and 366 nm. Absorption densitometry measured at 190 nm. Derivatization for peptides, amino acids and amino derivatives, by immersion into ninhydrin – collidine reagent (ninhydrin 0.3 %, collidine 5 %, acetic acid 5 %, in ethanol), followed by heating 5 min at 110 °C. Effect-directed analysis using automated immersion: A) for free radical (DPPH•) scavengers; B) for enzymatic inhibition (acetyl-cholinesterase, α-glucosidase); C) for activity against Gram-negative (Aliivibrio fischeri bioluminescence assay) or Gram-positive bacteria (Bacillus subtilis bioassay). Active bands were eluted with methanol through the oval elution head of a TLC-MS interface pump, into a quadrupole-Orbitrap mass spectrometer. Full scan mass spectra (m/z 200−2000) in positive and in negative ionization modes were recorded using heated electrospray ionization (HESI, spray voltage 3.5 kV, capillary temperature 270 °C). Active zones were assigned to be CLPs: iturin A, surfactin dimethyl-ester, and surfactin, fengycin and kurstakin homologues. Ex1 provided richer extracts compared to Ex2. Standards were seen to contain a free radical scavenging impurity.

      Classification: 4e, 8b, 18b, 23e
      129 064
      Effect-directed profiling and identification of bioactive metabolites from field, in vitro-grown and acclimatized Musa spp. accessions using high-performance thin-layer chromatography-mass spectrometry
      I.O. AYOOLA-ORESANYA, M.A. SONIBAREA, B. GUEYEB, R. PALIWALB, M.T. ABBERTON, Gertrud E. MORLOCK* (*Institute of Nutritional Science, and Interdisciplinary Research Centre for Biosystems, Land Use and Nutrition, Justus Liebig University Giessen, Giessen, Germany; gertrud.morlock@uni-giessen.de)

      J Chromatogr A, 1616, 460774 (2020). Methanolic extracts of leaves of Musa acuminata, M. balbisiana and M. sapientum (Musaceae), either from fields or from in vitro cultures or from the plantlets derived from in vitro culture and acclimatized in isolated warm room, were separated on HPTLC silica gel layers with toluene – ethyl acetate – methanol 6:3:1 or ethyl acetate – toluene – formic acid – water 34:5:7:5. When intended for MS experiments, layers were previously washed twice with methanol – formic acid 10:1, once with acetonitrile – methanol 2:1 and air-dried. Evaluation under white light, UV 254 nm and 366 nm. Derivatization by immersion (2s, 2cm/s) into natural product reagent preceded by heating at 110 °C for 5 min, or into anisaldehyde sulfuric acid reagent, diphenylamine aniline reagent, ninhydrin reagent, followed by the same heating procedure. Besides, plates were neutralized by cold air stream followed with phosphate buffer (8 %, pH 7.5) piezoelectrically sprayed on the plates and automated plate drying. Thereafter, 9 effect-directed assays (EDA) were performed for free radical (DPPH•) scavengers, for enzymatic inhibitors (α-amylase, acetyl- and butyryl-cholinesterase, α- and β-glucosidase), for antimicrobial compounds (Gram-positive Bacillus subtilis assay, Gram-negative Aliivibrio fischeri bioluminescence assay), and for mutagenic compounds (SOS response – UMU-C test using Salmonella typhimurium suspension and 4-nitroquinoline 1-oxide as positive control). The bands of 4 active compounds were eluted with methanol through a TLC-MS interface pump into a quadrupole-Orbitrap mass spectrometer. Full scan mass spectra (m/z 50−800) in the positive and negative ionization modes were recorded using electrospray ionization (ESI, spray voltage 3.3kV, capillary temperature 320°C, collision energy 35 eV). By comparison to a standard, one band present in all samples was identified as linolenic acid. For the other bands, only present in in vitro grown accessions, only raw molecular formulas and phytochemical classes were assigned (a pyrrolidine alkaloid, an amino-acid, a phenolic derivative).

      Classification: 4e, 7, 11a, 18a, 22, 32e
      128 043
      Nutritional and phytochemical profiling of nutracereal finger millet (Eleusine coracana L.) genotypes
      U. NAKARANI, D. SINGH*, K. SUTHAR, N. KARMAKAR, P. FALDU, H. PATIL (*Department of Plant Molecular Biology and Biotechnology, ACHF, NAU, Navsari, Gujarat 396 450, India, diwakar@nau.in)

      Food Chem. 341, 128271 (2021). HPTLC of finger millet (Eleusine coracana L.) on silica gel with n-butanol - water - acetic acid 4:1:1. Detection by spraying with ninhydrin, followed by heating at 100 °C. Amino acid profiling under UV light at 546 nm. The hRF values for 21 standard amino acids ranged from 2 to 51.

      Classification: 18a
      127 052
      Pressurized planar electrochromatography of DNS amino acids derivatives in silica gel and silanized silica gel systems with formic acid addition to the water mobile phase
      A. CHOMICKI*, T. DZIDO (*Department of Physical Chemistry, Medical University of Lublin, Chodźki 4a Str., 20-098 Lublin, Poland, adam.chomicki@umlub.pl)

      J. Planar Chromatogr. 34, 105-111 (2021). HPTLC of dansyl derivatives of amino acids on silica gel (1) and RP-18 (2) with acetonitrile in the concentration range from 0 to 40 % in water - formic acid solution for (1) and acetonitrile in the concentration range from 10 to 85 % in water - formic acid solution for (2). Pressurized planar electrochromatography (PPEC) under the same conditions with polarization voltage 0.500 kV and separation time of 15 min. Detection under UV light. The separation selectivity is different between HPTLC and PPEC due to the electrophoretic effect in PPEC.

      Classification: 18a
      127 002
      Low temperature plasma probe mass spectrometry for analytes separated on thin-layer chromatography plates: direct vs. laser assisted desorption.
      X. GONG, D. ZHANG, I. B. EMBILE, Y. SHE, S. SHI, G. GAMEZ* (*Department of Chemistry and Biochemistry, Texas Tech University, Lubbock, Texas, USA; gerardo.gamez@ttu.edu)

      J Am Soc Mass Spectrom 31(9), 1981-1993 (2020). Low-temperature plasma-mass spectrometry was studied for comparison between direct desorption (DD) and diode laser assisted desorption (LD) in terms of quantitative and qualitative analysis of compounds from cellulose vs. silica gel TLC layers. Compounds (the 20 common amino acids, propofol, nicotine, cotinine, salicylamide, acetylsalicylic acid, paracetamol, caffeine, valprolactone and its isomer 4-ene-valproic acid) were applied on the TLC plates (without development) at different concentrations; a commercial mixture of acetylsalicylic acid, paracetamol and caffeine was also applied on TLC plates, developed with dichloromethane – ethyl acetate 1:50, detection at UV 254 nm and quantitative MS. In general, DD provided good results on cellulose, where LODs where between 0.01 and 2.55 ng/mm2, whereas several compounds remained undetected on silica gel. LD however provided LODs on silica gel from 0.3 to 84 pg/mm2. Tandem MS with collision-induced dissociation was implemented to improve signals, LODs and to characterize the other analytical figures-of-merits (including detection of the main fragment ions, determination of optimal laser beam width and irradiance depending on the compounds). For the two metabolites of valproic acid, the ions and fragments had identical values; therefore, a mix of the two isomers had to be applied and separated with dichloromethane – methanol 50:1 before MS; one half of the plate was visualized for control by dipping into potassium permanganate reagent (7.5g KMnO4, 50g K2CO3, 0.75g NaOH in 1L water).

      Classification: 4e, 7, 8b, 11a, 18a, 22