优化分离与鉴定蓝斑背肛海兔口腔神经节蛋白质组

采用双向凝胶电泳技术优化分离蓝斑背肛海兔(Notarcus leachii cirrosus Stimpson, NLCS)口腔神经节(Buccal Ganglion, BG)蛋白质组, 并获得约300个蛋白质斑点. 用组合基质辅助激光解吸电离化飞行时间(MALDI-TOF)质谱技术和胶内酶解技术测定BG蛋白质组中的96个蛋白质斑点的肽指纹(Peptide mass fingerprint, PMF)图谱. 经数据库检索与比对后, 发现96种蛋白质中仅有4种蛋白质可获得较高的匹配率, 它们分别是微管蛋白(Tubulin)、 肌动蛋白(Actin)和两个1,5-二磷酸核酮糖-羧化酶/加氧酶(Ribulose-1,5-bisphosphate carboxylase/oxygenase, Ribulose), 均属于神经细胞骨架蛋白质; 同时还发现一种交配信号肽前体(Peptide mating pheromone precursor). 利用LOCtrees软件和分类法对56种蛋白质进行亚细胞定位与分类.     

Analysis of fragrances in cosmetics by gas chromatography–mass spectrometry

A gas chromatographic (GC)-mass spectrometric (GC-MS) method has been developed for the routine analysis of 11 fragrance substances in cosmetics: cinnamic alcohol, cinnamic aldehyde, eugenol, hydroxy citronellal, α-amyl cinnamic aldehyde, geraniol, isoeugenol, coumarin, dihydrocoumarin, citronellal and citral. Methods for sample preparation of various types of cosmetic products, prior to GC analysis, have also been developed and proved to be rugged. Detection limits of all of target fragrance substances were approximately 1 ppm. Calibration curves of the target fragrance substances analyzed by GC were found to be linear in the investigated concentration range, 0.005% – 0.50%. The recoveries of the target fragrances from various types of cosmetic products were 80% – 116% and the relative standard deviations of the quantitative analysis of the target fragrance substances were within 5%.     

Synthese,Struktur und Reaktivität von Bis(dialkylamino)diphosphanen

Synthesis, Structure, and Reactivity of Bis(dialkylamino)diphosphines Starting with the aminochlorophosphines ⁱPr₂N? PCl₂ 1 and (ⁱPr₂N)₂P? Cl 2 , the synthesis of some new functionalized aminophosphines (ⁱPr₂N)₂P? SiMe₃ 3a , (ⁱPr₂N)₂P? SnMe₃ 3b , (ⁱPr₂N)(DMP)P? Cl 4 , ⁱPr₂N? P(SiMe₃)₂ 5 and ⁱPr₂N? P(SiMe₃)Cl 6 is reported. Reactions of 2 with different phosphides yield the aminodiphosphines (ⁱPr₂N)₂P? P(SiMe₃)₂ 7a , (ⁱPr₂N)₂P? P(SiMe₂^tBu)₂ 7b , (ⁱPr₂N)₂P? PPh₂ 8 and (ⁱPr₂N)₂P? PH₂ 9 . The phosphines 3a/b react with halogenophosphines to the aminohalogenodiphosphines (ⁱPr₂N)₂P? PCl₂ 10 , (ⁱPr₂N)₂P? P^tBuCl 11 and (ⁱPr₂N)₂P? P(NⁱPr₂)Cl 12 . The ambivalente aminophosphine 6 gives the aminotrichlorodiphosphine Cl(ⁱPr₂N)P? PCl₂ 13 after condensation with PCl₃, while the reactions with the corresponding lithiumphosphides yield the aminosilyldiphosphines (ⁱPr₂N)(SiMe₃)P? P(SiMe₃)₂ 14a and (ⁱPr₂N)(SiMe₃)P? P(SiMe₂^tBu)₂ 14b . The aminochlorophosphines 2/4 are reductively coupled with magnesium leading to the symmetrically substituted tetraaminodiphosphines (ⁱPr₂N)₂P? P(ⁱPr₂N)₂ 15a and DMP(ⁱPr₂N)P? P(ⁱPr₂N)DMP 15b . The functionalized aminosilyldiphosphine 7a is treated with methanol to yield the diphosphine (ⁱPr₂N)₂P? PH(SiMe₃) 16 and gives the lithium phosphinophosphide (ⁱPr₂N)₂P? PLi(SiMe₃) 17 after metallation with n-BuLi. The compounds are characterized by their NMR and mass spectra and the ³¹P-NMR values of the diphosphines are discussed according to their substituents. The crystal structures of 7b, 8 and 15b showing significantly differing conformations are presented.     

Flavonoids in Leguminosae: analysis of extracts of T. pratense L., T. dubium L., T. repens L., and L. corniculatus L. leaves using liquid chromatography with UV, mass spectrometric and fluorescence detection

Reversed-phase LC on C-18 bonded silica with a methanol–ammonium formate gradient was used to determine the main flavonoids in leaves of four species of the Leguminosae family. The detection modes were diode-array UV absorbance, fluorescence, and (tandem) mass spectrometry. LC–UV was used for a general screening, sub-classification, and the calculation of total flavonoid contents. LC–FLU was included to identify isoflavones on the basis of their native fluorescence. Most structural information regarding aglycons, sugar moieties, and acidic groups was derived from LC–MS in both the full-scan and extracted-ion mode, using negative-ion atmospheric pressure chemical ionization. MS/MS did not provide much additional information, because the same fragments were observed as in full-scan MS.In T. pratense and T. repens, the main constituents were flavonoid glucoside–(di)malonates, while T. dubium and L. corniculatus mainly contained flavonoid (di)glycosides. Satellite sets comprising an aglycon, the glucoside and glucoside–malonates or –acetates, were abundantly present only in T. pratense. Generally speaking, the main aglycons and sugars in the four plant species are surprisingly different. In addition, while the results for T. pratense are similar to those reported in the literature, there is little agreement in the case of the other species. Finally, total flavonoid contents ranged from 50–65 mg/g for L. corniculatus and T. dubium, to 15 mg/g for T. pratense and only 1 mg/g for T. repens.     

Mass transfer determining parameter in facilitated transport through di-(2-ethylhexyl) dithiophosphoric acid activated composite membranes

Activated composite membranes (ACMs) containing di-(2-ethylhexyl) dithiophosphoric acid (D2EHDTPA) as a carrier have been found to facilitate the transport and separation of several cations. This paper describes an approach to the chemical characterisation of the transport phenomena of Zn²⁺, Cd²⁺, Cu²⁺, Ni²⁺, Sn²⁺ and In³⁺ by an ACM. The selectivity of D2EHDTPA based ACM towards different metal ions is presented and discussed focusing in Zn²⁺ and Cd²⁺ transport and recovery. Selectivity demonstrates that zinc ions are removable from mixtures due to the different extraction strength of D2EHDTPA. Such selectivity is based on the differences of the dynamic behaviour of the metal ions transport. In addition, a correlation of the chemical behaviour of those ACM systems with the corresponding solvent extraction systems has been found.     

Thermodynamic parameters of liquid ternary Fe1−x(Ni5/6Cr1/6)x alloys

Summary Computer-aidedKnudsen cell mass spectrometry is used for thermodynamic investigations on liquid ternary Fe_1–x(Ni_5/6Cr_1/6)_x alloys. The thermodynamic excess properties have been determined by means of the Digital Intensity-Ratio (DIR) method. Liquid ternary Fe_1–x(Ni_5/6Cr_1/6)_x alloys are characterized by exothermic molar heats of mixingH ^E, negative molar excessGibbs energiesG ^E, and negative molar excess entropiesS ^E. At 1850 K, the minimumH ^E value is –3120 J/mol (42.3 at.% Fe), the minimumG ^E value is –2540 J/mol (30 at.% Fe), and the minimumS ^E value is –0.44 J/(mol K) (60 at.% Fe). At 1850 K, the thermodynamic activities of Fe show slight negative deviations from the ideal behaviour for alloys with a Fe-content of less than 75 at.%, and ideal behaviour for the Fe-rich alloys (x _Fe>0.75).

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Thermodynamische Parameter flüssiger ternärer Fe_1–x(Ni_5/6Cr_1/6)_x-Legierungen

Zusammenfassung Die Thermodynamik flüssiger ternärer Fe_1–x(Ni_5/6Cr_1/6)_x-Legierungen wurde mit Hilfe der computerunterstützten Knudsenzellen-Massenspektrometrie studiert. Die thermodynamische Auswertung der experimentellen Untersuchungen erfolgte nach der digitalen Intensitätsverhältnismethode (DIR). Flüssige ternäre Fe_1–x(Ni_5/6Cr_1/6)_x-Legierungen zeigen exotherme molare MischungswärmenH ^E, negative molareGibbssche ZusatzenergienG ^E, und negative molare ZusatzentropienS ^E. Bei 1850 K sind die Minimumswerte fürH ^E –3120 J/mol (42.3 At.% Fe), fürG ^E –2540 J/mol (30 At.% Fe) und fürS ^E –0.44 J/(mol K) (60 At.% Fe). Bei 1850 K zeigen die thermodynamischen Aktivitäten von Fe bei Legierungen mit einem Fe-Gehalt von höchstens 75 At.% leichte negative Abweichungen vom idealen Verhalten, die Fe-reichsten Legierungen (x _Fe>0.75) verhalten sich hingegen nahezu ideal.

     

Komplexe von Vanadium und Titan mit Salicylaldehyd-benzoylhydrazon und 2-(2′-Hydroxyphenyl)-chinolin-8-ol. Kristallstruktur von μ-Oxo-bis[oxo{2-(2′-Hydroxyphenyl)-chinolin-8-olato(2-)}-vanadium(V)]

Complexes of Vanadium and Titanium with Salicylaldehyde benzoylhydrazone and 2-(2′-Hydroxyphenyl)-8-quinolinol. Crystal Structure of μ-Oxo-bis[oxo{2-(2′-hydroxyphenyl)-8-quinolinato(2-)}-vanadium(V)] . By reaction of titanium(IV)-isopropoxide and bis(acetylacetonato)-oxovanadium(IV) with salicylaldehyde benzoylhydrazone and 2-(2′hydroxyphenyl)-8-quinolinol, respectively, the metal complexes of the tridentate diacidic ligands were synthesized and characterized mass spectrometrically. The mass spectra of the titanium compounds correspond to the expected bisligand complexes whereas several species are demonstrable in the case of vanadium. Crystals of μ-oxo-bis[oxo{2-(2′-hydroxyphenyl)-8-quinolinolato(2-)}-vanadium(V)] were isolated and characterized by X-ray structural analysis. The complex exhibits C₂ symmetry, accordingly the μ₂-oxygen atom is situated on the 4 axis. The VOV bridge is angular with the unusually small bond angle of 107.3°. The coordination polyhedron is distorted octahedral. The compound additionally contains one molecule of chloroform per formula unit which is disordered in two positions. Crystallographic data see “Inhaltsübersicht”.     

Oral malodor,assessed by closed-loop,gas chromatography,and ion-trap technology

A method is described for the analysis of volatile organic compounds in saliva and tongue coating samples. The techniue is based on an off-line preconcentration step by means of a closed-loop trapping system followed by gas chromatography-ion trap detection. With the closed-loop technique, the volatile organic compounds(VOCs) are released from the matrix and trapped on an adsorbent without interference of water. The VOCs are released from the adsorbent into the gas chromatograph by thermdesorption. After separation, identification of the compounds is performed by ion trap technology. By this technique 82 compounds could be demonstrated in saliva and tongue coating samples. The technique is also used to demonstrate the formation of volatile bacterial fermentation compounds when a protein substrate is added to tongue coating samples. It is considered a very promising tool in further research on oral malodor.     

Direct coupling of polymer-based microchip electrophoresis to online MALDI-MS using a rotating ball inlet

We report on the coupling of a polymer-based microfluidic chip to a MALDI-TOF MS using a rotating ball interface. The microfluidic chips were fabricated by micromilling a mold insert into a brass plate, which was then used for replicating polymer microparts via hot embossing. Assembly of the chip was accomplished by thermally annealing a cover slip to the embossed substrate to enclose the channels. The linear separation channel was 50 microm wide, 100 microm deep, and possessed an 8 cm effective length separation channel with a double-T injector (V(inj) = 10 nL). The exit of the separation channel was machined to allow direct contact deposition of effluent onto a specially constructed rotating ball inlet to the mass spectrometer. Matrix addition was accomplished in-line on the surface of the ball. The coupling utilized the ball as the cathode transfer electrode to transport sample into the vacuum for desorption with a 355 nm Nd:YAG laser and analyzed on a TOF mass spectrometer. The ball was cleaned online after every rotation. The ability to couple poly(methylmethacrylate) microchip electrophoresis devices for the separation of peptides and peptide fragments produced from a protein digest with subsequent online MALDI MS detection was demonstrated.     

Towards molecular-imprint based SPE of local anaesthetics

Summary Solidago canadensis L., Canadian goldenrod (Asteraceae) has been used in European phytotheraphy for centuries as a component of urological and antiphlogistical remedies. High-performance liquid chromatography (HPLC) coupled with diode-array detection (DAD) and online mass spectrometry (MS) has been used for the separation and quantification of phenolics (chlorogenic acid, caffeic acid, kaempferol-3-O-α-L-rutinoside (nicotiflorin), quercetin-3-O-β-D-rutinoside (rutin), quercetin-3-O-β-D-galactoside (hyperoside), quercetin-3-O-β-D-glucoside (isoquercitrin), quercetin-3-O-β-D-rhamnoside (quercitrin), kaempferol-3-O-α-L-rhamnoside (afzelin) and quercetin from Solidaginis herba. Extracts have been obtained using different technologies. Three aqueous and three alcoholic extracts were studied separately. Reversedphase high-performance liquid chromatography separation of polyphenols on octadecyl sorbent Hypersil was performed, using acetonitrile: acetic acid 2.5 v/v % as eluent in gradient elution. Our results confirm previous reports concerning the presence of several flavonoids. Quantification of the main quercetin glycosides in pharmaceuticals is also reported. Presented at Balaton Symposium '01 on High-Performance Separation Methods, Siófok, Hungary, September 2–4, 2001