key: cord-0005146-jwhn09l7
authors: Wang, Jun; Lu, Ding-Qiang; Ling, Xiu-Quan; Wang, Jia-Li; Qiao, Hong-Qun; Ouyang, Ping-Kai
title: Simultaneous Determination of Four Active Components in Tobacco Wastes by LC
date: 2008-12-12
journal: Chromatographia
DOI: 10.1365/s10337-008-0908-8
sha: 57c290e6856e6e2a359b0cd928178ddda6a2332f
doc_id: 5146
cord_uid: jwhn09l7

A liquid chromatographic method was developed for the simultaneous quantification of four major active components in tobacco (Nicotiana tobaccum L.) wastes. Samples were extracted with 70% v/v aqueous methanol, four compounds including chlorogenic acid, cryptochlorogenic acid, neochlorogenic acid and caffeic acid were identified and determined by using LC coupled to electrospray tandem mass spectrometry and LC–UV method, respectively. Separation in LC–UV was on an Alltima C(18) column (250 mm × 4.6 mm i.d.; 5 μm) with a mobile phase consisting acetonitrile: ammonium acetate buffer (pH 4.5) (5:95 v/v), at a flow rate of 1.0 mL min(−1), detected at 327 nm. Four regression equations showed good linear relationships (r (2) > 0.999) between the peak area of each marker and concentration. The method has good repeatability and precision, the intra-day and inter-day RSD for both retention time and peak area was less than 1.0%. The recoveries, measured at three concentration levels, varied from 96.33 to 101.10%. The LOD (S/N = 3) and LOQ (S/N = 6) were less than 0.010 and 0.795 μg·mL(−1), respectively. This assay was successfully applied to the determination of four active compounds in ten samples. The results indicated that the developed assay method was rapid, accurate, reliable and could be readily utilized as a quantitative analysis method for various of tobacco wastes.

Tobacco (Nicotiana tobaccum L.) is widely grown as a non-food cash crop. As new relevant materials showed, China produced about 1840.5 million kg tobacco leaves in 2005 which amounts to 36.5% of the total output, and China has become the largest producing country in the world [1] . Tobacco leaves are mainly used for making cigarettes, cigars and for chewing. Large quantities of tobacco wastes are generated during processing and cigarette making which amounts to 25% of the total tobacco material, and China also has become the largest producing tobacco wastes country in the world. At the same time, disposal of these wastes is a serious problem nowadays, because tobacco wastes are toxic due to the presence of nicotine, and European Union Regulations (EUR) and Italian law classify tobacco wastes as ''toxic and hazardous wastes'' when the nicotine content exceeds 500 mg kg -1 dw [2] . However, besides nicotine, there are some other biologically important compounds in tobacco wastes, such as phenolic compounds [3] , solanesol [4] , transgenic proteins [5] , and so on. Recently, the chemical compositions of N. tabacum and tobacco wastes have attracted considerable attentions worldwide [3] , and tobacco wastes are considered to be a good source of a large number of bioactive substances. Moreover the report of utilization of solanesol from tobacco wastes [6] let us study the synthetic utilization of their active compounds, but not to degrade or discard them. In view of the potential pharmaceutical application, the identification of phenolic compounds from tobacco wastes is therefore of essential importance.

Phenolic compounds exist mostly in the form of glycosides or esters in living plants. They not only have important physiological and some pharmacological activities, but also influence the quality and property of some bioproducts [7] . Polyphenol compounds include tannins, coumarins, flavonols, anthocyanins, hydroxylated cyclohexanes and other phenol derivatives, which can affect the aroma of cigarettes, exist in tobacco (N.tabacum L.). Among them, chlorogonic acids and rutin are the most abundant polyphenols [8] . Unfortunately, less attention has been paid to the analysis and separation of phenolic compounds in tobacco wastes.

Chlorogenic acid is the only one compound in the large family, the best known conjugates are those with quinic acid, collectively known as chlorogenic acids (CGAs) or caffeoylquinic acids (CQAs) [9] . Classically, chlorogenic acids (CQAs) are a family of esters and related derivatives formed between certain trans cinnamic acids and (-)-quinic acid (1L-1(OH), 3,4,5-tetrahydroxycyclohexane carboxylic acid), the cinnamic acids most commonly encountered are caffeic, p-coumaric and ferulic [9, 10] . Compounds in this family possess a wide range of biological activities such as antibacterial, antioxidant, hepatocyte protective, antimutagenic, inhibition of HIV-1 RT and activities against human herpes simplex virus and adenoviruses, anti-SARS and anti-AIV(H5N1) activities [11] [12] [13] [14] [15] [16] [17] [18] . On the other hand, the tobacco manufacturing process and all the activities which use tobacco often produce tobacco wastes, and of the different solid wastes produced during the process. So, it is difficult to study the composition of CQAs in tobacco wastes. At the same time, profiling the phenolic compounds of tobacco wastes is important to the synthetic utilization of their active compounds.

Recently, LC-MS n has been used to characterize cinnamoylamino acid conjugates and to discriminate between individual isomers of mono-acyl and di-acyl chlorogenic acids [10, 19] , and also used to characterize flavanoids [20] . MS fragmentation data have been utilized to develop structure-diagnostic hierarchical keys for the identification of phenolic compounds. In this study, LC-MS was applied to the qualitative profiling of phenolic compounds such as chlorogenic acid (5-CQA), cryptochlorogenic acid (4-CQA), neochlorogenic acid (3-CQA) and caffeic acid (CA), see Fig. 1 ) in tobacco wastes. To enhance the separation of four compounds, a rapid, accurate and reliable LC-UV method was developed for the quantitative analysis of mark compounds in tobacco wastes samples.

The tobacco wastes were collected from various countries and regions in the world in 2007, and authenticated as the wastes of by Prof. Ding-qiang Lu (College of Life Science and Pharmaceutical Engineering, Nanjing University of Technology). Ten of these waste samples were dried at 60°C, powered by a herb disintegrator (Qinzhou Sanyang Package Equipment Co.) and then sieved (60 mesh).

LC-grade acetonitrile and acetic acid were purchased from TEDIA Co. (Fairfield, OH, USA); Chlorogenic acid (5-caffecylquinic acid, 5-CQA) and caffeic acid (CA) were purchased from the National Institute for the Control of Pharmaceutical and Biological Products (NICPBP), Beijing, China. Cryptochlorogenic acid (4-CQA) and neochlorogenic 

LC separation was performed on an Alltima C 18 (250 9 4.6 mm, 5 lm) column (Alltech, Deerfield, IL, USA). The mobile phase contained solvents A and B, where A was water: acetonitrile: acetic acid (97.5:2:0.5, v/v/v) and B was acetonitrile: acetic acid (99.5:0.5, v/v/v). The linear gradient profile was maintained 2% B in 5 min, from 2 to 5% in 5 min, from 5 to 10% in 20 min, from 10 to 35% in 35 min, from 35 to 100% in 15 min, from 100 to 2% in 5 min, and maintained 2% B in 5 min. The wavelength range of PAD detection was from 200 to 400 nm. The flow-rate was 1 mL min -1 for LC and PAD detection with the column kept at 40°C. A splitter was connected between the PAD and MS detectors, which reduced the flow rate to 0.2 mL min -1 for MS detection. The electrospray ESI-MS-ES was operated in the negative ion mode with scanning High purity nitrogen (99.9%) was used as dry gas to evaporate the solvent at a flow rate of 500 L h -1 at 350°C. Nitrogen was also used as nebuliser gas at 50 psi. LC-UV separation was performed on an Alltima C 18 (250 9 4.6 mm, 5 lm) column (Alltech). The mobile phase contained acetonitrile: ammonium acetate buffer (pH 4.5) (5:95, v/v). The flowrate was 1 mL min -1 and UV detection with the column kept at 30°C, detected at 327 nm.

The reference standards of the target compounds, i. e., 3-CQA, 4-CQA, 5-CQA and CA were accurately weighed, and their stock solution of 500, 450, 500 and 300 lg mL -1 concentration were prepared by dissolving in methanol, respectively. Then, the stock solutions were diluted to appropriate concentration ranges for the establishment of calibration curves. All solutions were stored at 4°C.

The powered samples (5.0 g) were extracted assisted by ultrasonic wave with 70% v/v aqueous methanol (125 mL) in an ultrasonic bath at 45°C for 45 min, to give an extraction yield of more than 70%. The extraction process was repeated two times, and the extract constant a volume of 500 mL. The obtained solutions were centrifuged at 10,000 rpm for 5 min, the supernatants were filtered through a 0.45 lm filter before injection. All samples were determined in triplicate.

LC chromatographic profiles of the 70% v/v aqueous methanol extract of tobacco wastes detected with negative ion mode ESI-MS and UV at 320 nm, see Fig. 1 .

In the methanolic extract of dried tobacco wastes, 3-CQA, 4-CQA, 5-CQA and CA were identified by comparing their retention times, UV (Fig. 1a) , ESI-TIC (Fig. 1b) , MS spectras and chemical structures (Fig.1c) with those of standard compounds. The structure of 3-CQA, 4-CQA, 5-CQA and CA were determined by MS SCAN model, and by comparing the UV and MS spectra data to those reported in the literature. These results show that CQAs in tobacco wastes are mainly composed of 3-CQA, 4-CQA, 5-CQA and CA.

In order to obtain optimal extraction, effect of extraction solvent, method, temperature and time on the extraction yield of active components from tobacco wastes were investigated. The results show that the extraction efficiency was highest when 70% methanol were used as solvent, ultrasonic-assisted extraction (UAE) was found to be more suitable than heat-reflux extraction (HRE) for the preparation of test samples, the optimal extraction temperature and solid-liquid ratio in UAE were 45°C and 1:25, respectively. The extraction yield of mark compounds was obtained almost 70% within 45 min in single-time extraction. Therefore, the optimal preparation method of four components in tobacco wastes were as follows: test samples were extracted with 70% v/v aqueous methanol by using UAE at 45°C for 45 min, which process was repeated twice.

To obtain chromatograms with a good separation and resolution of adjacent peaks within a short analysis time, mobile phase, column temperature and flow rate were optimized. The mobile phase containing acid, which could suppress the ionization of phenolic hydroxyl and carboxyl groups was beneficial for good retention and separation of chlorogenic, cryptochlorogenic, neochlorogenic and caffeic acids. Different mobile phase compositions (such as CH 3 

were attempted to separate the investigated four components. Acetonitrile:ammonium acetate buffer (pH 4.5) (5:95 v/v) was chosen as the eluting solvent system because efficient separation and desired peak shape could be achieved. Under isocratic elution modes, the four compounds could be separated effectively. The effect of temperature on the separation was investigated in the range of 25-40°C, 30°C was found to be optimal. The most suitable flow rate was found to be 1.0 mL min -1 . Since their polarity, solubility and other characteristics differ greatly; at least 15 min of elution time were needed for the simultaneous quantification of the four target compounds. On the basis of the UV-VIS spectra of the four components recorded by DAD detection in the range of 190-800 nm, experimental results indicate that four components have the same UV absorption peaks of about 327 nm, so 327 nm was selected for monitoring. Chromatograms of standard mixture (A) and tobacco wastes sample (B) are shown in Fig. 2 , peak shape of the four compounds in tobacco wastes were symmetrical. Under the optimized isocratic elution conditions chlorogenic acids and caffeic acid were separated with resolution greater than gradient elusion model. Each component in the samples analyzed was identified by comparing its retention time to that of the respective standard. Retention time for 3-CQA, 5-CQA, 4-CQA and CA were 4.9, 6.2, 7.4 and 11.3 min, respectively (see Fig. 2 ). Quantification was carried out by integration of the peaks using external standards. As shown in Fig. 2 , the LC-UV method was specific for separation of 3-CQA, 5-CQA, 4-CQA and CA in tobacco wastes.

Calibration curves were obtained by plotting peak areas versus six different concentrations of standard solutions. Response (peak area, Y) was then plotted against concentration (X, lg mL -1 ) and the six-point calibration curves were found to be linear as least squares regression gave a correlation coefficient. The equations were: neochlorogenic acid (3-CQA) Y = 6.196 9 10 7 X -4.453 9 10 4 (r 2 = 0.9997), chlorogenic acid (5-CQA) Y = 5.841 9 10 7 X -4.384 9 10 4 (r 2 = 0.9996), cryptochlorogenic acid (4-CQA) Y = 5.068 9 10 7 X -4.025 9 10 4 (r 2 = 0.9996), caffeic acid (CA) Y = 8.325 9 10 7 X -5.946 9 10 4 (r 2 = 0.9993), respectively.

The lowest acceptable level of the calibration curve was regarded as the limit of quantification (LOQ). The LOQ of neochlorogenic, chlorogenic, cryptochlorogenic and caffeic acids were 0.719, 0.751, 0.795 and 0.714 lg mL -1 , respectively. The limits of detection (LOD; S/N = 3) of neochlorogenic, chlorogenic, cryptochlorogenic and caffeic acids were 0.360, 0.376, 0.398 and 0.357 lg mL -1 , respectively. The LOD and LOQ values of the individual compound and the good linearity for each investigated compound indicated that the developed analytical method is precise and sensi- 

The repeatability of the method in the present work was examined by the intraday and inter-day variability. The intraday variability was examined on six individual samples within 1 day, and inter-day variability was determined for three different days. The relative standard deviation (RSD) was calculated as a measurement of method repeatability. The results shown in Table 1 indicated that the intra-and inter-day RSD values of the four marker compounds were less than 0.2%, which showed good reproducibility. The precision was evaluated using the results of five replicate injections of the standard solutions containing the four components. The results showed a good precision, and RSDs were less than 0.2%. For the stability test, the same sample solution was analyzed at different times within 48 h at room temperature. The RSD values of the peak areas were all lower than 1.0%, suggesting that it is safe to analyze the sample within 2 days.

Standard addition test was performed to determine the accuracy as well as the extraction recovery. In this test, the mixed standard solutions were prepared with three different concentration levels. 

The developed analytical method was successfully applied to the simultaneous determination of 3-CQA, 4-CQA, 5-CQA and CA in ten samples of tobacco wastes which were obtained from various countries and regions in the world, analysis results are listed in Table 2 .

As shown in Table 2 , the contents of four ingredients varied greatly among the different samples. In the majority of cases, 5-CQA was the main component, whose contents varied from 0.686 to 1.781% in ten samples, with almost 2.6-fold variation. Similar variation could also be found for the other components. The reason for the variation of the contents can be the difference of plant origin, the effect of environment and some other factors, such as season of collection, drying process and storage conditions, etc. Because variations of the marker compounds may influence the quality and potency of the tobacco wastes, it was necessary to develop an effective qualitative and quantitative method to evaluate the quality of tobacco wastes. The assay of one or two constituents only cannot give a complete assessment of the biomass. Thus, in this paper, four major compounds in tobacco wastes were analyzed simultaneously to evaluate its quality.

This is the first report on the simultaneous determination of neochlorogenic, chlorogenic, cryptochlorogenic and caffeic acids in tobacco wastes. The developed method was found to be rapid, linear, reliable and accurate. The validation procedure and assay results suggested that this LC-UV method is promising for being used in quality control of tobacco wastes.

Stud Nat Prod Chem (Bioactive Natural Products (Part F)