Container packed coffee beverage and process for production thereof

Information

  • Patent Application
  • 20080311271
  • Publication Number
    20080311271
  • Date Filed
    June 27, 2008
    16 years ago
  • Date Published
    December 18, 2008
    16 years ago
Abstract
A container-packed coffee beverage is provided, containing chlorogenic acids to a suitable extent, and furthermore having excellent taste, and with deterioration at heating has been suppressed. A container-packed coffee beverage containing the following constituents (A), (B) and (C): (A) Constituent α(B) Constituent β(C) chlorogenic acids wherein the peak area ratio of constituent (A) appearing in a retention time of 2.0 to 2.3 minutes and constituent (B) appearing in a retention time of 2.7 to 3.2 minutes on a chromatogram obtained by constituent analysis of a coffee extract at a detection wavelength of 260 nm using a high performance liquid chromatography apparatus is {(A)/(B)}×100=30 to 100, and the content ratio of 5-caffeoylquinic acid within the constituent (C) is 28.0 to 35.0% by weight, and a preparation method thereof is provided.
Description
TECHNICAL FIELD

The present invention relates to a container-packed coffee beverage containing chlorogenic acids to a suitable extent, and furthermore, having an excellent taste and whose deterioration at heating has been suppressed.


BACKGROUND ART

Coffee is a tasty beverage people enjoy drinking world-wide. In addition to conventional extraction from roasted beans and instant coffee, readily ingestible container-packed coffee beverages, are widely popular. In addition, useful constituents contained in coffee have been drawing attention in recent years. Chlorogenic acids are one among the useful constituents contained in coffee beverage. SOD-like activity is known as an effect of chlorogenic acids, reported to have the activity of suppressing the generation of reactive oxygen species and lipid peroxide involved in aging and a variety of sicknesses, and to have antioxidant activity (refer for instance to Japanese Patent Application Laid-open No. 2001-136910 and Japanese Patent Application Laid-open No. 2002-080351). The approximate amount of natural polyphenols such as chlorogenic acids to be ingested per day is 1 g per adult (refer for instance to Japanese Patent Application Laid-open No. 2005-312301), and simpler ingestion methods have been desired. As one such method, there is a method of increasing antioxidant activity by electrically processing the food source containing chlorogenic acids (refer for instance to Japanese Patent Application Laid-open No. 2003-102403).


In addition, among the chlorogenic acids, 3-caffeoylquinic acid, generally called neochlorogenic acid (refer for instance to Japanese Patent Application Laid-open No. 2004-033023), has been reported in particular to have an excellent antioxidant activity, and as simple ingestion methods thereof, there exist a method of separating chlorogenic acids by dextran gel to modify the mixing ratio (refer for instance to Japanese Patent Application Laid-open No. H09-143465) and a method of alkaline processing an aqueous solution containing chlorogenic acids (refer for instance to Japanese Patent Application Laid-open No. 2000-063827).


Elsewhere, 3-caffeoylquinic acid is known to be generated by heating 5-caffeoylquinic acid in alkali (refer for instance to “Quantification of chlorogenic acids and caffeine in coffee-containing beverage by high performance liquid chromatography” Takashi Ueki, Hiroshi Honda and Shiro Sakurai, Agricultural and Forestry Products Inspection Institute Issue No. 10, March 1986 (http://www.cfqlcs.go.jp/technical_information/investigation_research_report/rs10.htm).


In addition, chlorogenic acids are known to be in an unstable state when coffee beans are roasted, and that if heating history accumulates such as carrying out sterilization treatments on coffee extract, they decompose into small molecule organic acids, such as, acetic acid, formic acid, malic acid and citric acid, and as a result, sourness increases over time triggering deterioration (for instance Japanese Patent Application Laid-open No. H07-050993).


Meanwhile, there is q problem that when a container-packed beverage is heated at a store or in an automatic vending machine, the quality thereof remarkably deteriorates due to heating, and in order to solve this, for instance, a method of masking by adding flavor, or a method of adding cyclodextrin and ascorbic acid or ascorbic acid salt have been proposed (refer for instance to Japanese Patent Application Laid-open No. 2004-073057).


However, even if any of the above methods is selected, there are problems such as, caused by the addition of another constituent or carrying out special treatment subsequently to coffee beverage extraction; the original coffee taste is lost and the production cost increases due to the additional steps of production. In addition, since chlorogenic acids cause distracting flavors when contained in large quantities (refer for instance to Japanese Patent Application Laid-open No. 2005-333927, Japanese Patent Application Laid-open No. 2003-204755, Japanese Patent Application Laid-open No. 2003-204756), preserving the taste while leaving high concentrations of chlorogenic acids contained is difficult.


DISCLOSURE OF THE INVENTION

An object of the present invention is to provide a container-packed coffee beverage containing chlorogenic acids to a suitable extent, and furthermore, having an excellent taste and whose deterioration at heating has been suppressed.







BEST MODE FOR CARRYING OUT THE INVENTION

After earnest studies in order to resolve the above issues, the present inventors reached the ideas for the present invention. Specifically, the present inventors discovered that deterioration during heating of a container-packed coffee beverage could be suppressed by setting the content ratio of 5-caffeoylquinic acid among the chlorogenic acids within a specific range, and that taste could be improved by setting the peak area ratio of constituents α and β within a specific range.


More specifically, the present invention is as follows:


1. A container-packed coffee beverage containing the following constituents (A), (B) and (C):


(A) Peak α constituent


(B) Peak β constituent


(C) chlorogenic acids


wherein the peak area ratio of constituent (A) appearing in a retention time of 2.0 to 2.3 minutes and constituent (B) appearing in a retention time of 2.7 to 3.2 minutes on a chromatogram obtained by constituent analysis of a coffee extract at a detection wavelength of 260 nm using a high performance liquid chromatography apparatus is {(A)/(B)}×100=30 to 100, and the content ratio of 5-caffeoylquinic acid within the constituent (C) is 28.0 to 35.0% by weight.


2. In the above 1, a container-packed coffee beverage wherein the content in constituent (C) is 360 ppm or greater and 840 ppm or less in value converted into per 1.0% by weight of amount of solid coffee.


3. A method for preparing a container-packed coffee beverage, wherein adjustments are made in such a way that, in a coffee extract obtained by extracting coffee beans, the following constituents (A), (B) and (C) are contained:


(A) Peak α constituent


(B) Peak β constituent


(C) chlorogenic acids


and the peak area ratio of constituent (A) appearing in a retention time of 2.0 to 2.3 minutes and constituent (B) appearing in a retention time of 2.7 to 3.2 minutes on a chromatogram obtained by constituent analysis of a coffee extract at a detection wavelength of 260 nm using high performance liquid chromatography apparatus is {(A)/(B)}×100=30 to 100, and the content ratio of 5-caffeoylquinic acid within the constituent (C) is 28.0 to 35.0% by weight.


4. A method for preparing a container-packed coffee beverage, wherein for the adjustment in the above 3, roasted coffee beans having an L value of 16 to 21.5 and roasted coffee beans having an L value of 22 to 33 are blended at a ratio of 100:0 to 60:40.


5. A method for preparing a container-packed coffee beverage, wherein in the above 3 or 4, chlorogenic acids are added to the obtained coffee extract.


Hereinafter, embodiments of the present invention will be described. The terms used in the specification are defined as follows.


“(A) Peak α constituent” is an unidentified constituent, whose amount increases as the coffee beans are the more roasted; concretely, a constituent corresponding to peak obtained during constituent analysis of coffee extract using high performance liquid chromatography (HPLC), appearing at a detection wavelength of 260 nm and a retention time of 2.0 to 2.3 minute. The constituent can be measured by an HPLC apparatus. As HPLC apparatus, commercially available apparatus, for instance, “LaChrom” manufactured by Hitachi Ltd. and “LC-10A” manufactured by Shimadzu Corporation can be used; however, there are no particular limitations. The measurement conditions are set suitably so that the constituent can be detected. The column is not limited in particular as long as it can detect the constituent; however, the use of “inertsil ODS-2Φ3.0×250 mm” (manufactured by GL Sciences Inc.) is preferred.


“(B) Peak β constituent” is, in contrast to the α constituent, an unidentified constituent decreasing as coffee beans are more roasted, and can be measured by an HPLC apparatus under the same conditions as the α constituent. Concretely, it is a constituent corresponding to a peak obtained during constituent analysis of a coffee extract using an HPLC apparatus, appearing at a detection wavelength of 260 nm and a retention time of 2.7 to 3.2 minute.


In the specification, “(C) chlorogenic acids” is a collective term grouping 3-caffeoylquinic acid, 5-caffeoylquinic acid, 4-caffeoylquinic acid, 3-feruloylquinic acid, 5-feruloylquinic acid and 4-feruloylquinic acid. In addition, there are no particular limitations with respect to derivation thereof, and addition or elimination treatment may be carried out artificially.


“5-caffeoylquinic acid” is one of the constituents contained in constituent (C) chlorogenic acids. Weakest against heat among the chlorogenic acids, it has the property of either decomposing into small molecule organic acid, or isomerizing into 3-caffeoylquinic acid, as coffee beans are roasted. Therefore, the content in 5-caffeoylquinic acid varies during roasting of coffee beans, and the total amount of chlorogenic acids decreases as a result. In addition, although the antioxidant activity of the chlorogenic acids becomes higher when the content ratio of 3-caffeoylquinic acid rises due to the isomerization, if the content increases excessively the contribution of 3-caffeoylquinic acid to the antioxidant activity decreases. The small molecule organic acids generated by the decomposition of 5-caffeoylquinic acid have strong sourness and may become a cause of taste deterioration over time. Note that the deterioration is known to be attributable to generation of reactive oxygen species (radical). The higher the amount of radicals generated the more advanced the deterioration, and conversely, if the amount of radicals generated can be held down, the deterioration can be suppressed.


According to the present invention, by adjusting the above-mentioned four constituents to appropriate ranges, a container-packed coffee beverage can be obtained, containing chlorogenic acids to a suitable extent, and furthermore, having excellent taste and which deterioration at heating has been suppressed. From the viewpoints of chlorogenic acids amount and taste, the peak area ratio {(A)/(B)}×100 of (A) Constituent α and (B) Constituent β is adjusted to 30 to 100. Furthermore, in order to maintain an excellent taste, the adjustment is such that the ratio becomes 40 to 75, and preferably 50 to 65. The reasons are, at less than 30, a decrease in taste is observed, such as chlorogenic acids-derived distracting flavor becomes noticeable, and at 100 or greater, the amount of chlorogenic acids becomes excessively small.


From the viewpoints of quality and antioxidant activity, 360 ppm to 840 ppm, preferably 440 ppm to 710 ppm and more preferably 490 ppm to 600 ppm of chlorogenic acids (C) in values converted to per 1.0% by weight of amount of solid coffee may be contained. If 840 ppm is exceeded, care must be taken, as a large amount of chlorogenic acids decompose into small molecule organic acid due to heat, readily generating sourness, or the like, over time. From the amount of chlorogenic acids and the viewpoints of quality and antioxidant activity, the content ratio of 5-caffeoylquinic acid is adjusted to 28.0% to 35.0%, more preferably 28.8% to 31.5% and even more preferably 29.5% to 31.0%. At less than 28.0%, on top of the amount of chlorogenic acids becoming excessively small, the content ratio of 3-caffeoylquinic acid becomes excessively high, and contribution to antioxidant activity decreases. If 35.0% is exceeded, on top of the content ratio of 3-caffeoylquinic acid becomes small, and the antioxidant activity becoming low, sourness increases over time due to the content in 5-caffeoylquinic acid being high.


While the container-packed coffee beverage of the present invention can also be obtained by extracting roasted coffee beans in water or hot water by a conventional method, as the composition of the present invention is difficult to fulfill only with a single extract, it is preferably obtained by adjusting the constituents (A), (B) and (C) to give the previously mentioned composition, by blending of a plurality of extracts and/or addition of each constituent. For instance, deeply roasted coffee beans with an L value of 16 or greater and slightly roasted coffee beans with an L value of 33 or less may be blended at a ratio of 90:10 and extracted. In more detail, the L value of deeply roasted coffee beans is adjusted to 16 to 21.5, more preferably to 16.5 to 20, even more preferably to 17 to 19.5, and particularly preferably to 17.5 to 18.0. The L value of slightly roasted coffee beans is adjusted to 22 to 33, more preferably to 22.5 to 27, even more preferably to 23 to 26, and particularly preferably to 23.5 to 25.5. An object of the present invention is achieved by bringing the blending ratio to 100:0 to 60:40, more preferably to 95:5 to 70:30, and even more preferably to 90:10 to 80:20.


As places of production of coffee beans to be used, Brazil, Columbia, Tanzania, Mocha and the like can be cited, without any in particular restrictions. In addition, as bean product species, arabica species, robusta species, and the like may be cited. The coffee beans may be used as one species alone or by blending a plurality of species. Roasting is carried out using a general method, and the extent of roasting is adjusted suitably to obtain the extract necessary for the adjustment of each constituent. Concretely, bitterness becomes strong if roasting is deep and sourness becomes strong if roasting is slight.


The L value of the coffee beverage is preferably 28 to 62, more preferably 33 to 57, and even more preferably 38 to 52. Herein, an L value is a value that indicates luminosity. The L value of a coffee beverage can be measured according to common procedure using a colorimeter CT-310 (manufactured by Minolta) in a 1 cm cell.


The container-packed coffee beverage of the present invention can also be prepared by adding each constituent specified in the present invention alone. When adjusting the composition by adding chlorogenic acids alone, the addition of an extract of a plant containing chlorogenic acids is preferred. As plant raw materials containing chlorogenic acids that can be used herein, coffee (bean), howthorn, grape, Ligusticum wallichii, angelica acutiloba, coptis japonica, turmeric, asafoetida, sweet potato, molokheiya, sunflower (seed), apple (fruit), tobacco (leaf), pear (leaf), peach, and the like, may be cited. From the viewpoints of the taste of the coffee beverage, coffee extract is preferred. Furthermore, the coffee extract is preferably obtained from green coffee beans. Green coffee bean (i.e., raw coffee bean) extract can be obtained by grinding green coffee beans as necessary and extracting using ethanol, hydrous ethanol, methanol or the like, at a temperature of room temperature to 100° C. In addition a commercially available product, such as, flavor holder RC-30R, FH-1242, or the like, (Manufactured by T. Hasegawa Co., Ltd.) can also be used. In addition, when adding 5-caffeoylquinic acid alone, after grinding with sunflower seed as a material and extracting with water or hydrous alcohol, the obtained sunflower seed extract is adsorbed onto a styrene-divinyl benzene series porous polymerization resin, then eluted with an organic solvent such as methanol, the obtained chlorogenic acids-containing extract is further passed over a dextran gel-packed column and the eluate obtained by eluting with water can be used.


In addition, as desired, sugars, such as, sucrose, glucose, fructose, xylose, fructose-glucose solution and sugar alcohol, milk constituent, antioxidant, pH adjuster, emulsifier, flavor, and the like, can be added to the container-packed coffee beverage of the present invention. As milk constituents, raw milk, cow milk, whole dry milk, nonfat dry milk, raw cream, concentrated milk, nonfat milk, partially nonfat milk, condensed milk, and the like, may be cited. As the pH of the coffee beverage of the present invention, 3 to 7, furthermore 4 to 7, and in particular 5 to 7 are desirable from the aspect stability of the beverage.


As antioxidants, ascorbic acid or a salt thereof, erythorbic acid or a salt thereof, and the like, may be cited, among which, ascorbic acid or a salt thereof is particularly desirable.


As emulsifiers, sucrose fatty acid ester, glycerin fatty acid ester, microcrystal cellulose, lecithins, sorbitan fatty acid ester, polyglycerol fatty acid ester, and the like are preferred.


As containers used in the present invention, PET bottle, can (aluminum, steel), paper, retort pouch, bottle (glass), and the like, may be cited.


If heat sterilization is possible after filling into a container, as in the case of a metal can, sterilization treatment of coffee extract in the present invention is carried out under sterilization conditions defined in food sanitation law. Regarding those containers for which retort sterilization is not possible, such as PET bottle and paper container, methods such as sterilizing beforehand under equivalent sterilization conditions to conditions defined in the Food Sanitation Law, for instance, with a plate heat exchanger at high temperature and for a short-time, then cooling to a given temperature and filling a container, are adopted.


EXAMPLE

Hereinafter, the present invention will be described in further detail with examples; however, the scope of the present invention is not limited by these examples and the like.


[1. Analysis of Chlorogenic Acids and Constituents (α and β)]

The gradient elution method by HPLC was used as the method for analyzing chlorogenic acids and constituent (α and β). As the analyzer, Waters 2695 separation module (manufactured by Nihon Waters K.K.) was used as the HPLC main unit and Waters 2996 PDA (manufactured by Nihon Waters K.K.) was used as the detector. The analytical conditions were as follows:










TABLE 1







Column:
Inertsil ODS-2 φ3.0 × 250 mm


Mobile phase:


A Solution
3% acetonitrile solution containing 0.05 M acetic acid


B Solution
100% acetonitrile solution containing 0.05 M acetic



acid



Gradient elution method by (the program is shown



in Table 1)


Volume injected:
10 μL


Flow rate:
0.43 mL/min


Column
40 degree C.


temperature:










Detector: PDA UV 210 nm to 400 nm (retention time and detection wavelength of each constituent are shown in Table 2)












Gradient Program










(min)
Flow rate (mL)
A Solution (%)
B Solution (%)













INITIAL
1.0
100
0


 5.0
1.0
100
0


20.0
1.0
80
20


35.0
1.0
80
20


45.0
1.0
0
100


60.0
1.0
0
100


70.0
1.0
100
0


100.0 
1.0
100
0
















TABLE 2







Retention Time and Detection Wavelength










Retention time
Detection



(min)
wavelength













Chlorogenic acids




3-caffeoylquinic acid (3-CQA)
16.396
UV 325 nm


5-caffeoylquinic acid (5-CQA)
18.398
UV 325 nm


4-caffeoylquinic acid (4-CQA)
19.490
UV 325 nm


3-feruloylquinic acid (3-FQA)
20.204
UV 325 nm


5-feruloylquinic acid (5-FQA)
22.563
UV 325 nm


4-feruloylquinic acid (4-FQA)
23.267
UV 325 nm


Constituent


α constituent
2.217
UV 260 nm


β constituent
2.915
UV 260 nm









[(1)-1 Chlorogenic Acids Quantification Method]

Calibration Curve Construction Method:


Standards for 5-caffeoylquinic acid (5-CQA) (Manufactured by Wako Pure Chemical Industries Ltd.) were prepared with distilled water so as to yield three steps of concentrations in the order range of 20 ppm to 100 ppm to serve as standard solutions. A standard solution of each concentration was injected into the HPLC, and a three-point calibration curve was constructed from the peak area values and concentrations.


Sample Adjustment and Quantification Method:


Accurately, 5 mL of each sample was measured, placed in a 25 mL measuring flask, brought to a defined volume with distilled water, filtered with a 0.45 μm filter, and then injected into HPLC to quantify 5-CQA by the three-point calibration curve method mentioned previously. In addition, since no standard was available for the quantification of 3-caffeoylquinic acid (3-CQA), 4-caffeoylquinic acid (4-CQA), 3-feruloylquinic acid (3-FQA), 5-feruloylquinic acid (5-FQA) and 4-feruloylquinic acid (4-FQA), only qualification was carried out, the area value of each peak was calculated as an estimated value using the 5-CQA calibration curve, the total value of the 6 types chlorogenic acids was used as the amount of chlorogenic acids.


[(1)-2 Method for the Analysis of Constituents (α and β)]

Although constituents (α and β) are unidentified, the peak area value of each constituent was analyzed using the chromatogram at the detection wavelength of 260 nm obtained during (1)-1 Analysis of chlorogenic acids, and the area ratio (α/β value) determined by {area of α constituent/area of β constituent}×100 was calculated.









TABLE 3





















Regarding the α constituent, it became clear that it was a constituent detected in a retention time of 2.217 min under the HPLC conditions mentioned previously, with a maximum absorption wavelength of 257.9 nm, and increased by roasting. Regarding the β constituent, it became clear that it was a constituent detected in a retention time of 2.915 min under the HPLC conditions mentioned previously, with a maximum absorption wavelength of 263.8 nm and decreased by roasting. In Table 3, chromatograms at a detection wavelength of 260 nm are shown for coffee beverages test-produced with each raw material bean. At the top of Table 3, it is shown that a constituent and β constituent of a coffee beverage test-produced with slightly roasted beans, In the middle of Table 3, it is shown that α constituent and β constituent of a coffee beverage test-produced with medium roasted beans, and at the bottom of Table 3, it is shown that α constituent and β constituent of a coffee beverage test-produced with deeply roasted beans.


[(1)-3 Method for Measurement of Hydroxy Radical]

A radical (reactive oxygen species) is an index of quality deterioration, indicating the higher the quantity generated the more progressed the deterioration. For the method for measurement of hydroxy radical, each sample was heated at 60° C., and hydroxy radical generated at each time point was measured by the ESR method. (according to T. Am. Soc. Brew. Chem. 54 (4): 198-205, 205-211, 1996) For the reagent, spin trapping agent: PBN (N-tert-Butyl-α-phenylnitrone) (manufactured by Wako Pure Chemical Industries) was used, and the spin trapping agent reagent was prepared to 2.55M with 50% ethanol, 0.16 mL of which was added to 8 mL of sample and then stirred thoroughly. Heating was carried out at 60° C. with this solution in a thermostatic bath, hydroxy radical generated at each time was measured by the ESR, and the peak height of the hydroxy radical (PBN-OH) was calculated as a relative ratio against Mn (internal standard). ESR measurement conditions were as shown in Table 4. When the amount of radicals generated (relative ratio against Mn) is taken as the vertical axis and the heating time (min) is taken as the horizontal axis, the hydroxy radical generated when each sample was heated can be represented by an approximate linear equation having a certain slope, and the slope of this linear equation (radical generation velocity) was evaluated as the amount of radicals generated.












TABLE 4









Power
4 mW



ModWid
0.1 mT



C. Field
335.500 mT



Amp
1000



SwWid
(±) 5 mT



TimeC
1 sec



SwTime
4 min



Mn
550 nm










Example 1
Comparison of Coffee Beverages Test-Produced with Beans Having Different Degrees of Roasting

Chlorogenic acids content, area ratio of Constituents α and β, and amount of radicals generated at heating, of coffee beverages test-produced separately with coffee beans having different degrees of roasting were investigated.


A semi-hot air drum sample roaster having a 5 kg pan was used for roasting of coffee beans. After ignition to the burner, adjustment was made to medium heat, at the point where the internal temperature of the drum became 200° C., 3 kg of Brazil-produced beans were fed. While maintaining the heating power of the burner at medium heat, roasting was carried out until the target degree of roasting was reached, and after roasting, discharging and cooling were performed. The roasting time and drum internal temperature at discharge time for each roast bean used in the present test were as shown in Table 5. The roasted coffee beans were ground with a coffee cutter and the surface color was measured with the spectrophotometric colorimeter SE2000 from Nippon Denshoku Industries Co., Ltd.













TABLE 5









Discharge



L value
Roasting time
temperature



















Slight roast roasted coffee
32
10 minutes 00
190 degree C.


bean

seconds


Medium roast roasted coffee
21
11 minutes 50
200 degree C.


bean

seconds


Deep roast roasted coffee
17
12 minute 10
218 degree C.


bean

seconds









Extraction of coffee beverage was done by feeding 300 g of ground roasted coffee beans into a coffee extractor. After the bean surface was leveled, it was showered from the upper part of the extractor with hot water at 95° C., and after verifying that hot water penetrated the entirety of the beans, extract was recovered while continuing the showering.


Thereafter, the obtained extract was cooled to on the order of 30° C. in order to retain the quality. In addition, a flannel cloth was used to carry out filtration of the cooled extract to eliminate insoluble solid content of coffee. Finally, approximately 1500 g of extract was obtained, corresponding to a 5-fold amount with respect to coffee beans. The extraction efficiency estimate was 25%, and the time from the beginning of showering to the completion of extract recovery was 30 minutes.


The preparation of coffee extract was adjusted with distilled water so as to have an amount of solid coffee of 1.0% by weight, and 0.05% by weight of sodium bicarbonate was added simultaneously to adjust black coffee.


Filling and sterilization method was as follows; the prepared black coffee was heated to 90° C. then filled into a can, and seaming was carried out. Thereafter, retort sterilization was carried out under the conditions of 121° C. and 10 minutes.














TABLE 6












Amount of



Color of
Amount

radicals



material coffee beans
of

generated















L
L
L
chlorogenic

α/β*100
(slope of



value
value
value
acids
5-CQA/a*
(area
linear



32
21
17
(ppm)a
100 (%)
ratio)
equation)


















Sample 1
100%


1540 
32.9
 2.9
0.0482


Sample 2

100%

830
31.4
19.0
0.0173


Sample 3


100%
360
28.0
91.4
0.0050





















Amount of Radicals Generated During Heating of Each Coffee Beverage


From the results of Table 6, in the coffee beverages test-produced with raw material beans having different degrees of roasting, for sample 1 with slightly roasted beans as raw materials, the content in chlorogenic acids was high, and since there was little α constituent and abundant β constituent, the area ratio α/β value was a low value. In addition, for sample 1, the amount of radicals generated at heating was also found to be large. On the other hand, for sample 3 with deeply roasted beans as raw material, the content in chlorogenic acids decreased, and as α constituent increased and β constituent decreased, the area ratio α/β value was a higher value. In addition, for sample 3, the amount of radicals generated at heating was also found to be small.


Example 2
Comparison of Coffee Beverages Blending Coffee Beans Having Different Degrees of Roasting

Chlorogenic acids content, area ratio of Constituents α and β, and the amount of radicals generated at heating of coffee beverages test-produced by blending coffee beans having different degrees of roasting were investigated.


Green beans roasting method and coffee beverage preparation method were carried out by methods similar to Example 1. Coffee beans having different degrees of roasting were blended as described below, a coffee beverage was prepared by the preparation method of Example 1 such that the amount of solid coffee was 1.0% by weight, and the amount of chlorogenic acids, constituents (α and β), and the amount of radicals generated were investigated. The results are shown in Table 7.















TABLE 7













Amount of



Blending ratio of



radicals



material coffee
Amount of


generated



beans
chlorogenic

α/β*100
(slope of














L value
L value
acids
5-CQA/a*
(area
linear



32
17
(ppm)a
100 (%)
ratio)
equation)

















Sample 1
100% 
 0%
32.9
1540
2.9
0.0482


Sample 2
75%
25%
32.6
1230
12.2
0.0290


Sample 3
50%
50%
32.0
 930
25.9
0.0190


Sample 4
25%
75%
30.9
 630
47.5
0.0090


Sample 5
 0%
100% 
28.0
 360
91.4
0.0050





















Amount of Radicals Generated During Heating of Each Coffee Beverage


From the results of Table 7, also with coffee beverages blending raw material beans having different degrees of roasting, for samples 1 and 2 with high blending ratio of slightly roasted beans, the chlorogenic acid content was high and the area ratio of α constituent and β constituent had a low value. In addition, samples 1 and 2 were also found to have large amounts of radical generated at heating. On the other hand, for samples 4 and 5 with high blending ratio of deeply roasted beans, chlorogenic acids content was low, and the area ratio of α constituent and β constituent also had a high value. In addition, for samples 4 and 5, the amount of radicals generated at heating was also found to be lower. From these results, it was found that, in coffee beverages test-produced with coffee beans blending slightly roasted beans in abundance, the chlorogenic acids content was high, furthermore, the area ratio of α constituent and β constituent was low and the amount of radicals generated at heating was large.


Example 3
Relationship Between Chlorogenic Acids Content, α Constituent/β Constituent Area Ratio and Amount of Radicals Generated at Heating, and Sensory Evaluation after Heat Storage

The influence on the deterioration of quality after heat storage (at 70° C. for two weeks) exerted by the chlorogenic acids content, the area ratio of α constituent and β constituent, and the amount of radicals generated at heating of coffee beverages test-produced by blending different degrees of roasting raw material beans was investigated.


Green beans roasting method and coffee beverage preparation method were carried out by methods similar to Example 1. After storage at 70° C. for two weeks, sensory evaluation and a five-stage sourness intensity evaluation were carried out for each sample. Note that the sensory evaluation was carried out by five panelists who have excellent identification capabilities regarding coffee flavor.


Similarly to Example 2, coffee beans having different degrees of roasting were blended as shown in Table 8, a coffee beverage was prepared by the preparation method of Example 1 such that the amount of solid coffee was 1.0% by weight, and the amount of chlorogenic acids, constituents (α and β), and the amount of radicals generated were investigated.















TABLE 8













Amount of



Blending ratio of



radicals



material coffee beans
Amount of


generated
















L
L
L
L
chlorogenic
5-CQA/
α/β*100
(slope of



value
value
value
value
acids
a*100
(area
linear



32
17
16
15
(ppm)a
(%)
ratio)
equation)



















Sample 1
75%
25%


1230 
32.6
12.2
0.0290


Sample 2
50%
50%


970
32.0
23.7
0.0190


Sample 3
40%
60%


840
31.6
30.8
0.0130


Sample 4
30%
70%


710
31.4
40.5
0.0078


Sample 5
20%
80%


600
30.7
49.4
0.0084


Sample 6
10%
90%


490
29.5
62.2
0.0081


Sample 7
 5%
95%


440
28.8
72.2
0.0070


Sample 8
 0%
 5%


360
28.0
91.4
0.0050


Sample 9


100%

230
25.2
150.2
0.0043


Sample 10



100%
140
24.8
247.7
0.0044







































TABLE 9









Overall



Sensory evaluation
Sourness intensity
evaluation



















Sample 1
Strong fermentation odor,
0.25
X



abundant distracting flavors


Sample 2
Fermentation-like
0.25
X



deterioration odor


Sample 3
Somewhat fermentation-like
1.38




deterioration odor


Sample 4
Somewhat fermentation-like
1.25




deterioration odor


Sample 5
Weakest sourness
1.75



Sample 6
Weakest sourness
2.00



Sample 7
Somewhat strong sourness
2.13



Sample 8
Strong sourness
2.50



Sample 9
Strong sourness and
3.00
X



abundant distracting flavors


Sample 10
Abundant distracting flavors
2.75
X



and burnt odor sensed









From the results of Table 8 and Table 9, similarly as before, with coffee beverages blending coffee beans having different degrees of roasting, when the blending ratio of slightly roasted beans became higher, the chlorogenic acids content was high and the area ratio of α constituent and β constituent had a low value. In addition, amount of radicals generated at heating also became large when the blending ratio of slightly roasted beans became higher. On the other hand, when the blending ratio of deeply roasted beans became higher, chlorogenic acids content was low and the area ratio of α constituent and β constituent had also a high value. In addition, the amount of radicals generated at heating also became low when the blending ratio of deeply roasted beans became higher.


Resulting from the sensory evaluation after conservation at 70° C. for two weeks, for samples 1 and 2 with high blending ratio of slightly roasted beans, fermentation-like deterioration odor could be strongly sensed, and for sample 1 distracting flavor could also be sensed abundantly. On the other hand, for samples 9 and 10, in which deeply roasted beans with a strong degree of roasting were used, distracting flavor, burnt odor, sourness and the like, were strongly sensed, and for sample 8, sourness was also sensed strongly. From the above results, it was thought that, when the blending ratio of slightly roasted beans became higher, chlorogenic acids content became large and the amount of radicals generated, which are considered to be one of the causes of deterioration, also became large, deterioration due to heat storage occurred, and fermentation odor and the like could be sensed strongly. In addition, with deeply roasted beans, if the degree of roasting became strong, the amount of chlorogenic acids became low and the amount of radicals generated also became low; however, after heat storage, distracting flavor, burnt taste, sourness and the like, tended to be stronger. From the above results, sample 3 to sample 8 had satisfactory sensory evaluation and good overall evaluation.


Example 4
Comparison Between Coffee Beverage Test-Produced with Medium Roasted Beans and Coffee Beverage Blending Slightly Roasted Beans and Deeply Roasted Beans

The amount of radicals generated at heating and the situation of quality deterioration after heat storage (at 70° C. for two week) of coffee beverage from medium roasted beans and coffee beverage blending slightly roasted beans and deeply roasted beans with the same extent in chlorogenic acids content were investigated.


Green beans roasting method and coffee beverage preparation method were carried out by methods similar to Example 1. Sensory evaluation method was carried out by a similar method to Example 3.


Similarly to Example 2, coffee beans having different degrees of roasting were blended as shown in Table 10, a coffee beverage was prepared by the preparation method of Example 1 such that the amount of solid coffee was 1.0% by weight, and the amount of chlorogenic acids, constituents (α and β), and the amount of radicals generated were investigated.















TABLE 10









Blending ratio of



Amount of



material coffee beans
Amount of

α/β*10
radicals
















L
L
L
L
chlorogenic
5-CQA/
0
generated



value
value
value
value
acids
a*100
(area
(slope of



32
25
20
17
(ppm)a
(%)
ratio)
linear equation)



















Sample 1


100%

760
30.0
28.4
0.0099


Sample 2
20%


80%
730
30.2
37.9
0.0105


Sample 3

100%


1330
33.1
5.8
0.0416


Sample 4
50%


50%
1070
31.5
20.5
0.0183
















TABLE 11







Sensory evaluation results and sourness intensity after storage


at 70° C. for two weeks












Sourness
Overall



Sensory evaluation
intensity
evaluation














Sample 1
Somewhat sourness taste sensed,
3.00
X



abundant distracting flavors,



strong sourness


Sample 2
Somewhat sourness taste sensed
2.00




but satisfactory flavor and also



has bitterness


Sample 3
Grainy taste sensed, abundant
2.25
X



distracting flavors, strong



sourness


Sample 4
Distracting flavors somewhat
1.25
X



present, fermentation-like



deterioration odor









From the results of Table 10 and Table 11, samples 1 and 3 test-produced with medium roasted beans alone had graininess, and distracting flavor, sourness and the like could be sensed strongly; however, by blending deeply roasted beans and slightly roasted beans, for sample 2, deeply roasted beans-derived bitterness could be sensed and the flavor was satisfactory. Consequently, even with the same extent of chlorogenic acids concentration, blending deeply roasted beans and slightly roasted beans gave satisfactory flavor and stability after heat storage. However, for sample 4, with a high blending ratio of slightly roasted beans and large amount of chlorogenic acids, fermentation odor could be sensed.


INDUSTRIAL APPLICABILITY

According to the present invention, by giving the above-mentioned composition, a container-packed coffee beverage, can be provided, having an excellent taste while containing chlorogenic acids to a suitable extent, which are useful constituents found in coffee, and furthermore, whose deterioration at heating has been suppressed.

Claims
  • 1. A container-packed coffee beverage containing the following constituents (A), (B) and (C): (A) Peak α constituent(B) Peak β constituent(C) chlorogenic acids
  • 2. The container-packed coffee beverage as recited in claim 1, the content in said constituent (C) is 360 ppm or greater and 840 ppm or less in value converted into per 1.0% by weight of amount of solid coffee.
  • 3. A method for preparing a container-packed coffee beverage, wherein adjustments are made in such a way that, in a coffee extract obtained by extracting coffee beans, the following constituents (A), (B) and (C) are contained: (A) Peak α constituent(B) Peak β constituent(C) chlorogenic acids
  • 4. The method for preparing a container-packed coffee beverage as recited in claim 3, wherein for said adjustment, roasted coffee beans having an L value of 16 to 21.5 and roasted coffee beans having an L value of 22 to 33 are blended at a ratio of 100:0 to 60:40 to obtain a coffee extract.
  • 5. The method for preparing a container-packed coffee beverage as recited in claim 3 or 4, wherein chlorogenic acids are added to said obtained coffee extract.
Priority Claims (1)
Number Date Country Kind
2005-380686 Dec 2005 JP national
Continuation in Parts (1)
Number Date Country
Parent PCT/JP2006/025445 Dec 2006 US
Child 12216045 US