Introduction
Coffee is one of the most commercialized agricultural products in the world and consumed by its pleasant aroma that together with its stimulating effect generate great acceptability in the population (Yener et al., 2015). When making a coffee infusion, a variety of chemical compounds responsible for their sensorial quality are extracted, including lipids, which are rich in diterpenes, sterols, tocopherols, phosphatides and waxes (Tryptamine derivatives (Villarreal et al., 2012; Ferrari et al., 2010)). The extraction depends on the temperature, water chemistry and the accessible coffee surface area (Uman et al., 2016). In the coffee non-saponifiable fraction, the diterpenes (Kahweol & cafestol Dias et al., 2013).
Among the methods to obtain the roasted coffee lipid fraction, are the extraction with solvent and supercritical fluid (Hurtado et al., 2016). The coffee lipid fraction constitutes 11 to 20% of green grain, depending on the variety (Al-Hamamre et al., 2010). Intake of lipids from coffee infusions is not a significant source of fat in the human diet, 0.4 g has been reported in five unfiltered daily infusions (Budryn et al., 2012).
These variations in quality are influenced by the availability of oxygen, moisture, exposed surface and temperature in the roasting processes (Pérez-Martínez et al., 2008).
During the coffee grain roasting, these formed carbonyl compounds can react with amino groups and form Schiff bases (Maillard reaction), besides reactions such as depolymerization, pyrolysis, Strecker reaction among others. Some coffee lipid compounds have been used as chemotaxonomic markers. Fatty acids have become chemical descriptors used to differentiate among coffee varieties. Sterols have been used as suitable markers for coffee blending studies (Speer & Kölling-Speer, 2006).
It has been shown that arabica coffee grains cultivated at altitudes between 1020-1200 m. a. s. l., have a positive effect on the final beverage quality, although there is a great dependence on the crop site of origin (Avelino et al., 2005). The chlorogenic acid and fatty acid contents in seeds depend on air temperature, contrary to total lipids, total soluble sugars and polysaccharides in coffee seed, which were not influenced by the climate (Joët et al., 2010). Thus, continuing studies on vegetable lipids (Murcia et al., 2013), The aim of the present research was to Characterize chemically, physically and sensorially samples of coffee (Coffea arábica var. caturra) Roasted and ground cultivated in three altitudinal ranges (1300-1400, 1400-1600, 1600-1800 m. a. s. l.) in coffee farms of the municipality of Pitalito, department of Huila, Colombia.
Materials and methods
Sample collection and treatment
Samples of cherry coffee (Coffea arábica var. Caturra), were supplied by farmers from nine farms with commercial coffee plantations in the rural area of the municipality of Pitalito, south side of Huila department, Colombia, in the corregimientos of Brussels and Palestine. The coffee farms were coded as J1, J2 and J3 for the altitudinal range of 1300-1400 m. a. s. l., J4, J5 & J6 for the altitudinal range of 1400-1600 m. a. s. l. and J7, J8 & J9 for the altitudinal range of 1600-1800 m. a. s. l. and selected according to availability of coffee grain for the present study. The samples were pulped using a mechanical demucilaginator and sun-dried on terraces at an ambient temperature between 25-28 ° C, obtaining the dried Pergamino coffee grains. Samples of dried Pergamino coffee, were stored at a temperature of 18-21° C in dark plastic bag. The husk was extracted to the Pergamino coffee grains with the Quantik C-200 thresher and they were toasted in a Quantik TC150AR kiln following the protocol of the Association of Special Coffees of America up to a medium roasting level with an L value of 21, 43 (obtained from the mixture of nine J1-J9replicates), corresponding to a degree of clear-medium roasting.
Physical, chemical and sensory analysis
In samples of dry Pergamino coffee grains, moisture was measured by the Quantik MH-302 hygrometer before and during roasting, initial temperature (°C), final temperature (°C), cracking time (seconds), total time (seconds) and color, using Quantik IR800 digital colorimeter. Titratable acidity was determined (NTC 5247), pH (Potentiometry, Pereira et al., 2007) and lipid fraction (Soxhlet, Martín et al., 2001). Subsequently, this lipid fraction was mixed with KOH/2N MeOH. The reaction mixture was extracted with benzene and dried with anhydrous sodium sulfate prior to GC-MS analysis considering the methodology suggested by Díaz & Vásquez (2011).
Sensory analysis was performed with the application of the SCAA protocol (Toledo et al., 2016), by Q-grader tasting panel and sensorial attributes were determined as follows: fragrance/aroma, taste, residual taste, acidity, body, uniformity, balance, clean cup, sweetness and final score. Tasting table was composed by twelve coffee samples (two cups per sample) and were presented only with their codes. The tasting results were recorded in the SCAA format. The final score was calculated by summing the individual scores given for each of the aforementioned attributes and using the quality classification of coffee according to the total score as follows: 90-100% (exceptional), 85-89,99% (excellent), 80-84,99 (very good) y <80,0% Lower than the special quality.
Gas chromatography of high resolution - Mass spectrometry of electronic impact (GC-EI)
GC-EI analysis of the extracted organic phase with benzene was carried out on a gas chromatograph with mass selective detector (Shimadzu QP-2010) in scan mode. The automatic injector system AOC-20i, autosampler with injection AOC-20s splitless, direct injection system controlled by computer software. An Agilent HP-5 (5% of fenilmetilsiloxan) capillary column was used with 30 m length and 320 μm of internal diameter and 0.25 μm of film thickness. The entrainment gas used was high purity Helium with a constant flow of 1mL.min-1. The temperature in the injector and the detector was 350 ° C in each case.
Statistic analysis
For each of the chemical compounds identified by (GC-EI) and sensory attributes of cup quality were performed descriptive statistics (means and variable frequencies) and a means analysis using the Tukey test P˂0.05). A principal component analysis was performed (PCA) and Partial least squares regression PLS (Partial Least Squares) using the graphic option of Scatterplot Matrix to find the relationships between the compounds identified in the lipid fraction of Coffea arábica var. caturra and sensory attributes using the R software version 3.2.3.(r), Throughout the independent platform for statistical analysis R Commander, based on the package FactoMineR(r).
Results and discussion
Physical and chemical characteristics of coffee samples
Table 1, shows the results of physicochemical analysis of ground and roasted Caturra coffee variety samples. The average moisture contents of the dried Pergamino coffee before roasting to different altitudinal ranges studied were as follows: 16.1 ± 4.90% (Coefficient of variation: 30.4) in the altitudinal range of 1300-1400 m. a. s. l. 7.97 ± 2.67 (33.5) in the altitudinal range of 1400-1600 m. a. s. l. and 8.9 ± 1.0 (11.2) in the altitudinal range of 1600-1800 m. a. s. l., there was a significant difference (P˂0.05) among moisture values of the dry Pergamino coffee samples of the altitudinal range 1300-1400 m. a. s. l. with respect to the other two evaluated altitudinal ranges: 1400-1600 and 1600-1800 m. a. s. l. (which did not present significant difference (p>0.05) each other). The moisture content of the ground and roasted coffee samples from the three altitudinal ranges evaluated in the present study ranged from 0.773 to 1.031%, with no significant difference (p<0.05) among altitudinal ranges. These moisture values are below the maximum allowable moisture value for roasted and ground coffee (<5%) Given by the Colombian technical standard NTC 3534.
*Cracking time: Period of time in which the grain begins to grow and begins to take brown color during the roasting. ** Roasting with open doors. a Different lowercase letter to the right of the coefficient of variation (CV) in the same row indicates significant difference (p<0.05).wb: Wet basis; db: Dry basis.
The sensorial attributes evaluated in the cup test of samples of roasted and ground coffee evaluated here, presented total scores between 82.8 & 83.4, which are associated with very good qualification regardless of the considered altitude (Table 3). Budryn et al. (2012), indicated the roasting range of 190 to 216°C, Provides acceptable sensory properties to coffee. In this research was verified the decreasing values of the roasting range to values of 162.3- 200.7°C (Table 1), also a product of very good quality is achieved considering the total scores obtained (Table 3).
The range found for the total lipid content of roasted and ground coffee was 11.5 and 12.1 % on a dry basis (Table 1), lower than found for other coffee growing areas in Brazil (13.5% accordingly to Ferrari et al., 2010), 15% in accordance with Calligaris et al. (2009), and India (15.28% accordingly to Al-Hamamre et al., 2010; 16.5-16.4% in accordance with Ferrari et al., 2010), these variations are largely due to differences in geographical conditions (Avelino et al., 2005).
The pH values found here were as follows: 5.2-5.3 (Table 1) and are among the optimum range for ground and roasted grains worldwide (5.1- 5.8). The cause of the decrease in pH values is due to the increase of organic acids (formic, acetic, glycolic and lactic acid) produced by thermooxidation processes.
The acidity values found were as follows: 21.5 ± 1.57 to 23.9 ± 3.39 mg of clorogenic acid. g of coffee-1 (Table 1) Being greater than those described for medium dark roasted coffee C. arabica cv. Bourbon in Brazil (10.8), C. arabica cv. Long Berry in Etiophy (9.4) and C. canephora cv. robusta in Uganda (13.34) (Farah et al., 2005).
Composition of the unsaponifiable fraction of Coffea arabica var. caturra
According to the analysis of GC-EI mass spectra, twelve compounds were identified in the non-saponifiable lipid fraction of roasted and ground coffee (Table 2), predominating stigmasterol, beta-sitosterol and 4-methylpentanamide in the three evaluated altitudinal ranges. On the other hand, it was observed that as the altitudinal range increases, the content of 4-methylpentanamide and phytol decreases, as well as the content of 2-ethenyl-1,3,5-trimethylbenzene, allyl-tolyl ether and 4-methyl- 2H-benzopyran (Table 2). Alil or-tolil eter only showed significant difference between the altitudinal ranges of 1400-1600 and 1600-1800 m. a. s. l. These compounds found, for the most part, are products of lipid degradation in this type of sample (Caldeira & Bassoli, 2007).
4-Methyl-2H-benzopyran was identified at altitudes 1400-1600 and 1600-1800 m. a. s. l., this type of compound has been registered in roasted coffee, whose nucleus is part of the flavonoids structure and it is common to find it in samples of roasted coffee (Farah, 2005). In roasted coffee, nitrogenous rings such as pyridine, pyrazine and pyrrole are more common when working at roasting temperatures between 210-230°C (Toledo et al., 2016).
In the present research, stigmasterol and beta-sitosterol were registered, two common sterols in coffee samples, which coincides with studies of sterols in roasted and ground Coffea arabica cultivated in United States (ɣ-sitosterol 53% and estigmasterol 21%). The stigmasterol contents of the present research (Table 2) Are higher than the values reported in tasting coffee lipids and consumption type of C. arabica var. Colombia (6.5%) obtained by supercritical fluid (Días & Vásquez, 2011). In addition, 2-propenamide (acrylamide), a nitrogen compound which occurs during the Maillard reaction, is identified in the coffee roasting process (Alves et al., 2009).
Butanal has been described as the product of the oxidative thermo-degradation of linoleic acid found in coffee samples. Finally, the presence of phytol, diterpene, which is part of the chlorophyll structure and found in lipid fractions of this type of samples (Siriamornpun et al., 2014).
Chromatographic profile comparison of the unsaponifiable fraction according to the altitudinal range
According to the non-saponifiable fraction chromatography profiles of ground and roasted coffee lipids of C. arabica (Figure 1), the relative abundances of some compounds, which varied were analyzed according to the altitudinal range. To 1300-1400 and 1400-1600 m. a. s. l., predominance of the 4-metilpentanamide (4), 2-(2-Hidroxifenil) buta-1,3-dieno (7), and beta sitosterol (12) compounds. Contrary to what was found for the altitudinal range of 1600-1800 m. a. s. l., in repetitions J7 and J8, where there was a slight predominance of 2-etenil-1,3,5-trimetilbenzene (6), estigmasterol (11) and beta-sitosterol (12) compounds.
From each altitudinal range, three replicates of ground and roasted coffee samples were used as follows: 1300-1400 m (J1, J2 and J3), 1400-1600 m. a. s. l., (J4, J5 and J6) and 1600-1800 m. a. s. l. (J7, J8 and J9). Chromatographic peaks: (1) 2-propenamide, (2) Butanal, (3) 1-propenilaziridine, (4) 4-metilpentanamide, (5) 3-fenil-2-propenal, (6) 2-etenil-1,3-5-trimetilbenzene, (7) 2-(2-hidroxifenil)buta-1,3-dieno, (8) alil o-tolil eter, (9) 4-metil-2H-benzopirane, (10) fitol, (11) estigmasterol and (12) beta sitosterol.
The J9 sample of ground coffee roasted from the altitudinal range of 1600-1800 m. a. s. l., performed a different chromatographic profile compared to J7 and J8 and with respect to repetitions (J1 to J6) from other altitudinal ranges considered (Figure 1). It is likely the J9 repetition has been contaminated with another species or coffee variety, for example, Coffea canephora var. robusta, cultivar preferred by some coffee growers in the study area. It is to denote the physical and chemical variables determined in samples of C. arabica var caturra ground and roasted including J9 repetition at different altitudinal range 1600-1800 m. a. s. l., showed no significant difference with the altitudinal ranges of 1300-1400 and 1600-1800 m. a. s. l. (Table 1). Likewise, similar values were presented in attributes of the cup quality test (Table 3), Varying the altitudinal range and within the range of 1600-1800 m. a. s. l., including J9 repetition. It is noteworthy that differences were observed with respect to qualities and notes between repetitions J2 to J9 in the tasting test (Table 4) Indicating the relative abundance of the same compound in different replicates (J2 to J9), generates different sensory attributes (notes and qualities) in tasting test (Table 4). In conclusion, the chromatographic profiles of the non-saponifiable fraction of ground coffee and roasted coffee C. arabica are very similar between replicates and the three evaluated altitudinal ranges (Figure 1), except for J9 repetition, which is most likely according to the respective chromatographic profile to be contaminated with another variety of coffee as suggested above.
Sensorial analysis
The sensory attributes of the evaluated samples (replicates) from C. arabica var. Caturra, did not vary between different altitudinal ranges (Table 3), but there were different and specific notes and qualities for each J2-J9 repetition (Table 4). Butanal, found in the present research and its derivatives have been associated with negative earthy notes, which decrease the drink quality. Butanal derivatives, generally of San Salvador carbonyl compounds are associated with aromas described as fatty, dairy and greenish. The presence of butanal and alkylbenzenes (i.e. metilbenzene,1,3-bis-1,1-dimetiletilbenzene (possibly 2-etenil-1,3,5-trimetilbenzene), are associated with crude defective seeds (Toledo et al., 2016). The butanal presence could be related to the very good qualification of coffee quality evaluated in the present research according to total score (Table 3). In the attributes quantitative descriptive analysis, was evidenced that uniformity, clean cup and sweetness were the attributes which obtained the highest score in the cup quality test independent of the evaluated altitudinal range (Figure 2). On the other hand, a slightly higher total score was observed in the cup quality test (total score 83.4%), in samples of C. arabica var caturra cultivated to 1600-1800 m. a. s. l. with notes of papaya and qualities like raspberry, blackberry, lemon malt, panela and melon (Table 4), which showed higher allyl-tolyl ether and 4-methyl-2H-benzopyran contents compared to the other evaluated altitudinal ranges (Table 2).
m±ds(cv)= Mean ± standard deviation (coefficient of variation). MM: molar mass, CAS: chemical abstract service. a different lowercase letters to the right of the standard deviation (sd) In the same row indicates significant difference (p<0.05)
Relationship between chromatographic profile and sensory analysis
The first two components of PCA explains (3-phenyl-2-propenal, 2-ethenyl-1,3,5-trimethylbenzene, 3-phenyl-2-propenal), the main relationship was presented for fragrance/aroma and body, Allyl-tolyl ether, Figure 3). The relationships between compounds identified in the lipid fraction of Coffea arábica var. caturra and sensorial attributes, which were obtained from different groupings in relation to the coefficients of correlation magnitude with fragrance/aroma between 3-fenil-2-Propenal, (r2:0.81 P˂0.01, Figure 4a), 2-etenil-1,3,5-trimetilbenzene (r2:0.6743 P˂0.01, Figure 4b) and alil o-tolil eter (r2:0.6343 P˂0.01, Figure 4c). The body showed correlation with 2-etenil-1,3,5-trimetilbenzene (r2:0.5409 P˂0.01, Figure 4d), 2-(2-Hidroxifenil)buta-1,3-dieno (r2:0.5363 P˂0.01, Figure 4e) and alil o-tolil eter (r2:0.5014 P˂0.01, Figure 4f).
Conclusion
In the non-saponifiable fraction of C. arabica var. Caturra, to three altitudinal ranges, was tentatively determined: 2-propenamida, Butanal, 1-propenilaziridine, 4-metilpentanamide, 3-fenil-2-propenal, 2-etenil-1,3-5-trimetilbenzene, 2-(2-hidroxifenil)buta-1,3-dieno, alil o-tolil eter, 4-metil-2H-benzopirane, fitol, estigmasterol and beta sitosterol. The sensorial attributes evaluated in the cup test of samples of roasted and ground coffee evaluated here, presented very good qualification regardless of the considered altitude. Chromatographic profiles of the unsaponifiable fraction of ground and roasted coffee C. arabica are very similar between replicates and the three evaluated altitudinal ranges. The butanal presence and 3-phenyl-2-propenal, could explain the low grade obtained by coffee samples in the cup quality test in the group of special coffees.