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Title:
METHOD OF RESOLVING ALLERGENS IN PERFUME INGREDIENTS
Document Type and Number:
WIPO Patent Application WO/2017/207467
Kind Code:
A1
Abstract:
Analytical methods that can be employed to reliably separate known or suspected allergens in a complex mixture of fragrance ingredients are described.

Inventors:
DUTRIEZ THOMAS (FR)
OWEN NEIL (GB)
Application Number:
PCT/EP2017/062853
Publication Date:
December 07, 2017
Filing Date:
May 29, 2017
Export Citation:
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Assignee:
GIVAUDAN SA (CH)
International Classes:
G01N30/46; C11B9/00; G01N30/86; G06F19/00
Foreign References:
US20150299614A12015-10-22
Other References:
CHIARA CORDERO ET AL: "Evaluation of different internal-diameter column combinations in comprehensive two-dimensional gas chromatography in flavour and fragrance analysis", JOURNAL OF SEPARATION SCIENCE., vol. 31, no. 19, 16 October 2008 (2008-10-16), DE, pages 3437 - 3450, XP055402481, ISSN: 1615-9306, DOI: 10.1002/jssc.200800280
LAURE MAHÉ ET AL: "Global approach for the selection of high temperature comprehensive two-dimensional gas chromatography experimental conditions and quantitative analysis in regards to sulfur-containing compounds in heavy petroleum cuts", JOURNAL OF CHROMATOGRAPHY A, vol. 1218, no. 3, 3 December 2010 (2010-12-03) - 21 January 2011 (2011-01-21), AMSTERDAM, NL, pages 534 - 544, XP055402646, ISSN: 0021-9673, DOI: 10.1016/j.chroma.2010.11.065
IAN D. WILSON: "Encyclopedia of Separation Science", 2000, ELSEVIER, ISBN: 978-0-12-2267, article MARRIOTT ET AL.: "Multidimensional Gas Chromatography", pages: 536 - 544
L.M. BLUMBERG ET AL., J. CHROMATOGR. A, vol. 1188, 2008, pages 2 - 16
L.M. BLUMBERG ET AL., J. SEP. SCI., vol. 31, 2008, pages 3352 - 3357
G. PURCARO ET AL., ANAL. CHEM., vol. 82, 2010, pages 8583 - 8590
M. S. DUNN ET AL., J. CHROM. A, vol. 1130, 2006, pages 122 - 129
H. LEIJS ET AL., J. AGRIC. FOOD CHEM., vol. 53, 2005, pages 5487 - 5491
C. CORDERO ET AL., J. CHROM. A, vol. 1150, 2007, pages 37 - 49
R. SHELLIE ET AL., FLAVOUR FRAGR. J., vol. 19, 2004, pages 91 - 98
CORTES H.J.: "Multidimensional Chromatography: Techniques and Applications", 1990, MARCEL DEKKER, article J.C. GIDDINGS: "Multidimensional Chromatography: Techniques and Applications"
L.M. BLUMBERG ET AL., J. SEP. SCI, vol. 31, 2008, pages 3352 - 3357
KLEE ET AL., J. CHROM. A, vol. 1383, 2015, pages 151 - 9
LAN ET AL., ANAL. CHEM., vol. 71, 1999, pages 709 - 714
F. BERTONCINI, M. COURTIADE-THOLANCE, D. THIEBAUT: "Gas Chromatography and 2D-GC chromatography for petroleum industry", 2013, EDITIONS TECHNIP., article T. DUTRIEZ: "GCxGC: a disruptive technique", pages: 46
S. BOUCHONNET: "Introduction to GC-MS Coupling", 2013, CRC PRESS
Attorney, Agent or Firm:
GLOBAL PATENTS (CH)
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Claims:
CLAIMS

A method of resolving defined known or suspected allergens in a complex mixture of perfume ingredients using two-dimensional gas chromatography, wherein the combination of first and second stationary phases is selected on the basis of a clustering analysis of defined known or suspected allergens providing a Separation Efficiency parameter (SE2D) of 94% or greater wherein

and wherein s2D is the two-dimensional resolution between two neighbouring peaks (a) and (b), corresponding to two different defined known or suspected allergens on a 2D-GC contour plot, given by the formula: and wherein

Mr is the average number of time each peak is sampled by the modulator, rounded upper value,

PM is the 2D-GC modulation period in seconds, Aztr is the difference of retention times between two neighbouring peaks (a) and (b) on the first dimension (x-axis);

Δ tr js difference of retention times between the same two neighbouring peaks (a) and (b) on the second dimension (y-axis); FlV/-//-/0 is the second dimension peak width of a peak (a) at half height and 2FWHHb is the second dimension peak width of a peak (b) at half height; two defined known or suspected allergens having an Rs2D value of 1 or higher are well separated and are referred to as Singletons (S); and two defined known or suspected allergens having an s2D value of less than cluster; and wherein n is the number of Singletons (S); m is the number of defined known or suspected allergens belonging to a cluster; o is the number of clusters for a given known or suspected allergens; and Rs2D ; is the Rs2D value for a defined analytical target /' in a given cluster j.

A method according to claim 1 wherein the first stationary phase has an intermediate polarity, and the second stationary phase is relatively polar compared with the first stationary phase.

A method according to claim 2 wherein the first stationary phase is an arylene-modified diphenyl-dimethyl siloxane copolymer stationary phase.

A method according to claim 3 wherein arylene-modified diphenyl-dimethyl siloxane copolymer comprises 20 to about 60 wt% diphenylsiloxane moieties and about 40 to about 80 wt% arylene dimethyl siloxane moieties, more particularly from about 30 to about 40 wt% diphenylsiloxane groups and from about 60 to 70 wt% arylene dimethyl siloxane moieties, and still more particularly from about 33 to about 38 wt% diphenylsiloxane moieties and from about 62 to about 67 wt% arylene dimethyl siloxane moieties , wherein the weight percentage (wt%) is relative to the total weight of the copolymer.

A method according to claim 3 wherein arylene-modified diphenyl-dimethyl siloxane copolymer is a copolymer comprising about 35% diphenylsiloxane moieties and about 65% dimethylsiloxane and arylene dimethyl siloxane moieties

A method according to any of the preceding claims wherein the second stationary phase is a (polyethylene-glycol) wax.

A method according to any of the preceding claims wherein the known or suspected allergen is selected from the group consisting of Acetyl Cedrene (main isomer) (32388-55- 9 ); Alpha Isomethylionone (127-51-5); Amyl Cinnamic Alcohol (E) (101-85-9); Amyl Cinnamic Aldehyde (E) (122-40-7); Amyl Salicylate (ISO-) (87-20-7); Amyl Salicylate (N-) (2050-08-0); Anethole Trans (E) (4180-23-8); Anisyl Alcohol (105-13-5); Benzaldehyde (100-52-7); Benzyl Alcohol (100-51-6); Benzyl Benzoate (120-51-4); Benzyl Cinnamate (E) (103-41-3); Benzyl Cyanide (140-29-4); Benzyl Salicylate (118-58-1); Camphor (76-22-2); Carvone (99-49-0); Caryophyllene Beta (87-44-5); Cinnamic Alcohol (E) (104-54-1); Cinnamic Aldehyde (E) (104-55-2); Citronellol (106-22-9); Coumarin (91-64-5); Hydroxyisohexyl 3-cyclohexene carboxaldehyde (Cyclohexal / Lyral major) (31906-04-4); Hydroxyisohexyl 3-cyclohexene carboxaldehyde (Cyclohexal / Lyral minor) (51414-25-6); Damascenone Beta (23696-85-7); Damascone Alpha (E) (24720-09-0); Damascone Alpha (Z) (23726-94-5); Damascone Beta (E) (23726-91-2); Damascone Beta (Z) (23726-92-3 ); Damascone Delta cis/trans (71048-83-4); Damascone Delta trans/cis (n/a); Damascone Delta trans/trans (71048-82-3); Di Iso-Butyl Phthalate (84-69-5); Di isopentyl phthalate (605-50-5 ); Di Isopropyl Phthalate (605-45-8); Di n-Butyl Phthalate (84-74-2); Di n-pentyl phthalate (131-18-0 ); Dicyclohexyl phthalate (84-61-7 ); Diethyl Hexyl Phthalate (117-81- 7); Diethyl Phthalate (84-66-2); Dimethyl Phthalate (131-11-3); Dimethyl Benzyl Carbinyl Acetate (151-05-3); Ebanol 1 (67801-20-1); Ebanol 2 (67801-20-1); Estragol (140-67-0); Eugenol (97-53-0); Eugenyl acetate (93-28-7); Farnesol (E)(E) (106-28-5); Farnesol (Z)(E) (3790-71-4); Farnesol (E)(Z) (3879-60-5); Farnesol (Z)(Z) (16106-95-9); Galaxolide (Cis) (252933-49-6); Galaxolide (Trans) (252933-48-5); Geranial (141-27-5); Geraniol (106-24- 1); Geranyl Acetate (105-87-3); Hexadecanolide (109-29-5); Hexyl Cinnamic Aldehyde (E) (101-86-0); Hydroxycitronellal (107-75-5); Iso E Super Alpha (68155-66-8); Iso E Super Beta (54464-57-2); Iso E Super Gamma (68155-67-9); Iso E Super minor (54464-59-4); Isoeugenol (E) (5932-68-3); Isoeugenol (Z) (5912-86-7); Isoeugenyl Acetate (93-29-8); Lilial (80-54-6); Limonene (5989-27-5); Linalool (78-70-6); Linalyl Acetate (115-95-7); Majantol (103694-68-4); Menthol (1490-04-6); Methoxycoumarin-7 (531-59-9 ); Methyl Eugenol (93-15-2); Methyl Heptine Carbonate (111-12-6); Methyl Octine Carbonate (111-80-8); Methyl Salicylate (119-36-8); Neral (106-26-3); n-pentyl isopentyl phthalate (84777-06-0 ); Phenyl Acetaldehyde (122-78-1); Pinene Alpha (80-56-8); Pinene Beta (127-91-3); Propylidene Phthalide 3- (E) (56014-72-3); Propylidene Phthalide 3- (Z) (94704-89-9); Salicylaldehyde (90-02-8); Santalol Alpha (115-71-9); Santalol Beta (77-42-9); Sclareol (515-03-7); Terpinene Alpha (99-86-5); Terpineol Alpha (98-55-5); Terpineol Beta cis (7299-41-4); Terpineol Beta trans (7299-40-3); Terpineol Delta (7299-42-5); Terpineol Gamma (586-81-2); Terpinolene (586-62-9); and Vanillin (121-33-5).

8. A method according to any of the preceding claims, wherein the complex mixture of perfume ingredients comprises at least one known or suspected allergen as defined in claim 6.

9. A method of preparing a perfume composition comprising the step of including in said 5 composition at least one perfume ingredient that is either not a defined known or suspected allergen, or is an ingredient that is substantially free of defined known or suspected allergens, as determined by two-dimensional gas chromatography, wherein the combination of stationary phases for two-dimensional comprehensive gas chromatography are selected on the basis of a method as defined in any of the claims 1 10 through 7.

10. A consumer product composition comprising a perfume composition as defined in claim 8.

11. A consumer product composition according to claim 9 selected from a leave-on or rinse- off personal care or cosmetic composition.

15 12. A leave-on composition according to claim 10 characterized in that if any known or suspected allergens as defined in claim 6 are present in said composition none are present in amounts exceeding 10 ppm as determined by a method according to any of the claims 1 through 7.

13. A rinse-off composition according to claim 10 characterized in that if any known or 20 suspected allergens as defined in claim 6 are present in said composition none are present in amounts exceeding 100 ppm as determined by a method according to any of the claims 1 through 7.

Description:
METHOD OF RESOLVING ALLERGENS IN PERFUME INGREDIENTS

Field of the invention

This disclosure is related to a method of detecting analytical targets, such as known or suspected allergenic compounds, in complex mixtures of ingredients, and in particular complex mixtures of fragrance ingredients. It is also related to a method of preparing complex mixtures, and particularly fragrance compositions, that are free or substantially free of said analytical targets, particularly known or suspected allergenic compounds, and to complex mixtures prepared by said method.

Background of the invention Fragrance compositions used in both fine perfumery and functional perfumery very often consist of complex mixtures that may contain tens or even hundreds of fragrance ingredients. Furthermore, some fragrance ingredients that are considered to be single ingredients from the perspective of a perfumer (such as essential oils) may actually contain many hundreds of components and impurities, some of which may be considered to be potentially allergenic substances within the terms of the 7 th Amendment of the Cosmetics Directive, Directive 2003/15/EC.

Indeed, currently, there are 24 ingredients that are categorized as potential allergenic substances under the Directive, and the possibility cannot be discounted that more substances will be similarly categorized in the future. For companies desirous of adding fragrance compositions to personal care or cosmetic products , it will be important to know if those fragrance compositions contain significant levels of any impurities that may be considered to be potential allergenic compounds under the Directive.

Chromatographic techniques are already well known in the art for separating complex mixtures. Most high resolution gas chromatography techniques have been developed to separate aliphatic and aromatic hydrocarbons. However, chemical compounds that have pleasant odours and which are therefore interesting as perfume ingredients tend to possess substantially similar chemical and physical properties, such as molecular weight, polarity and the like. And because of these similar properties, potentially allergenic ingredients contained in complex fragrance compositions, may be difficult to resolve and quantify analytically. New and higher resolution analytical approaches, characterized by stringent prerequisites in terms of analytical resolution and selectivity are required.

Comprehensive two-dimensional chromatography, also referred to as GCxGC or 2D-GC in the literature, is a known method for separating complex mixtures of analytes. In GCxGC, a complex 5 mixture is separated on a first capillary column comprising a first stationary phase 1 D before being separated a second time, portion wise, on a second capillary column comprising a second stationary phase 2 D, see for example Marriott et al., "Multidimensional Gas Chromatography" in "Encyclopedia of Separation Science, Ian D. Wilson (Editor), Elsevier, 2000, ISBN: 978-0-12- 226770-3, pages 536-544.

10 The main advantage of comprehensive two-dimensional chromatography over conventional high resolution chromatography is its much higher peak capacity, which may be 9 to 11 times larger than that of the latter. The term "peak capacity" describes the number of peaks that can be fitted on to a chromatogram between two defined points, each peak being separated from its neighbour by a defined amount. Theoretically, maximum peak capacity is achieved when two

15 stationary phases are orthogonal, that is, the mechanisms of separation in two dimensions are independent of each other. For this reason, it is customary to use combinations of polar x apolar or apolar x polar columns.

Peak capacity is commonly used to assess the quality of a stationary phase or of a combination of stationary phases, and optimization of the performance of chromatographic separation process 20 commonly involves maximizing the peak capacity (see for example L.M. Blumberg et al., J.

Chromatogr. A 1188 (2008) 2-16. L.M. Blumberg et al., J. Sep. Sci. 31 (2008) 3352-3357). Selection of stationary phases is typically based on an optimization of peak capacity, and the process is iterative and can be laborious.

The use of GCxGC method for determining the composition of complex mixtures, such as natural 25 essential oils is known. In recent years, several authors have attempted to use this method to resolve and then quantify a limited number of potentially allergenic substances that may be present in such essential oils: see for example G. Purcaro et al. Anal. Chem. 2010, 82, 8583-8590; M. S. Dunn et al. J. Chrom. A, 1130 (2006) 122-129; H. Leijs et al. J. Agric. Food Chem. 2005, 53, 5487-5491; C. Cordero et al. J. Chrom. A, 1150 (2007) 37-49; . Shellie et al. Flavour Fragr. J. 30 2004; 19: 91-98. However, in all these studies, the number of suspected allergens that has been separated and then quantified was limited to 24. Although it has been possible to overcome the problem of separating the current list of 24 of suspected allergens, existing techniques are insufficient in regard to the increasing number of substances that are suspected to be potentially allergenic, and which may come under scrutiny by regulatory authorities. Indeed, a new extended list of suspected allergens and regulated substances has been drawn up, comprising 95 substances, set forth in Table 1 below.

The principal limitation with previous attempts to achieve such complex separation tasks lies in the systematic selection of a first apolar stationary phase and, in most cases, selection of a second polar phase to maximize the difference of polarity between both stationary phases. Typically, a first, apolar stationary phase comprising 95% and more poly(dimethyl-siloxane) combined with a second, polar stationary phase comprising polyethylene glycol, or a second intermediate polarity stationary phase were used. In one case, the first stationary phase was a 100% poly(dimethyl- siloxane) apolar phase and the second stationary phase had an intermediate polarity (C. Cordero et al. J. Chrom. A, 1150 (2007) 37-49). However the applicant found that these particular combinations of stationary phase were unable to resolve a mixture containing the extended list of substances.

However, applicant systematically examined and found that conventional 2D-GC set-ups combining a first apolar column with a second polar column, or a first apolar column with a second mid polar column, or a first polar column and a second apolar column, did not provide the desired 2D separation efficiency of mixtures containing the extended list of substances.

Applicant has found that relying on peak capacity to select the combined stationary phases in a comprehensive two-dimensional gas chromatography set-up was not sufficient for achieving the analytical resolution required to separate the aforementioned complex mixture set forth in Table 1. A high peak capacity will inform an analyst that a particular column selection is likely to increase the chance of a reasonable separation, but it will not predict that separation will be optimal for a given complex mixture.

Absent reliable and accurate analytical data regarding the presence of the 95 known or suspected allergens that may be found in fragrance compositions, consumers may have insufficient information to be sure of satisfying requirements of any existing or upcoming regulation. But beyond any consideration of regulatory issues, existing analytical techniques are simply inadequate for the skilled person to resolve and eventually quanitify individual known or suspected allergens in complex mixtures of fragrance ingredients.

There remains a need to provide analytical methods that can be employed to reliably separate known or suspected allergens in a complex mixtures of fragrance ingredients, and thereby enable further identification and quantification of these allergens.

Summary of the invention

The applicant has now found a novel stationary phase selection criterion, based on clustering analysis of a group of defined analytical targets, which criterion is defined hereunder as the two- dimensional separation efficiency (SE 2D ). Stationary phase combinations that in a 2D-GC set up will score a SE 2D value above a threshold value, defined hereinbelow, will separate with good resolution said defined group of analytical targets.

The invention provides in a first aspect, a method of selecting combinations of stationary phases for two-dimensional comprehensive gas chromatography of a complex mixture, the selection being based on a Separation Efficiency parameter SE 2D , derived from a clustering analysis of defined analytical targets.

The invention provides in another aspect a method of resolving defined analytical targets in a complex mixture using two-dimensional gas chromatography, wherein the combination of stationary phases for two-dimensional comprehensive gas chromatography are selected on the basis of a Separation Efficiency parameter SE 2D , derived from a clustering analysis of defined analytical targets.

In another aspect of the invention there is provided a method of preparing a composition comprising the step of including in said composition at least one ingredient that is either not a defined analytical target, or is an ingredient that is substantially free of defined analytical targets, as determined by two-dimensional comprehensive gas chromatography, wherein the combination of stationary phases for two-dimensional comprehensive gas chromatography are selected on the basis of a Separation Efficiency parameter SE 2D , derived from a clustering analysis of defined analytical targets.

In yet another aspect of the invention there is provided a composition that is substantially free of defined analytical targets, as determined by two-dimensional comprehensive gas chromatography, wherein the combination of stationary phases for two-dimensional comprehensive gas chromatography are selected on the basis of a Separation Efficiency parameter SE 2D , derived from a clustering analysis of defined analytical targets.

DETAILED DESCRIPTION OF THE INVENTION The present invention is based on a clustering analysis of defined analytical targets. The clustering analysis is described more fully hereinbelow. Although the invention is applicable to the separation of any defined analytical targets contained in a complex mixture in order that they can be identified and/or quantified as required, the invention is hereinafter illustrated with particular reference to a group of defined analytical targets consisting of a list of 95 known or suspected allergens set forth hereinbelow in Table 1.

If a 2D-GC set up contains a combination of stationary phases that delivers a Separation Efficiency (SE 2D ) value above a certain threshold value defined hereinbelow, then the individual known or suspected allergens can be satisfactorily separated in a mixture containing all 95 of said allergens. And it follows from this that said allergens could be identified, and ultimately separated and quantified from a complex mixture of fragrance ingredients, using techniques known in the art.

The methodology of the present invention is based on a novel metric for assessing the resolving power of a 2D-GC set-up based on a defined list of known or suspected allergens involving a clustering analysis of neighbouring peaks having a known mutual two-dimensional resolution value Rs 2D , which is defined hereunder. The methodology is further characterized in that the clustering behaviour of the defined known or suspected allergens is based on the value of the mutual two-dimensional resolution, wherein two known or suspected allergens having mutual two-dimensional resolution (Rs 2D ) value of 1 or higher are considered to be well separated, whereas two known or suspected allergens having mutual two-dimensional resolution (Rs 2D ) value lower than 1 are not considered to be well separated, and therefore belong to the same cluster.

The mutual two dimensional resolution Rs 2D is defined as the two-dimensional resolution between two neighbouring peaks, corresponding to two different defined analytical targets, on a 2D-GC contour plot, as shown in Figure 1, and is expressed by the following equation, see J.C. Giddings, Multidimensional Chromatography: Techniques and Applications. In: Multidimensional Chromatography: Techniques and Applicati ons (Cortes H.J. Ed) , Marcel Dekker, New York (1990), which is hereby incorporated by reference.

Rs, Equation 1 wherein

A l tr is the difference of retention times between two neighbouring peaks (a) and (b) on the first dimension (x-axis);

A 2 tr is the difference of retention times between the same two neighbouring peaks (a) and (b) on the second dimension (y-axis);

ιω α is the first dimension 6σ peak width of the peak (a) (on x-axis);

lco b is the first dimension 6σ peak width of peak (b) (on x-axis);

2 oo a is the second dimension 6σ peak width of the peak (a) (on y-axis); and

2 > b is the second dimension 6σ peak width of the peak (b) (on y-axis). As a particularly useful approximation, the applicant has, however, found that equation above could be simplified into the following equation

2 xA l tr V f 2 xA 2 tr

Rs, +

2 x (M r + l) x P h M J 2.55 x( 2 FWHH a + FWHH h ) Equation 2

where

M r is the average number of times each peak is sampled by the modulator, as described hereunder, rounded to the upper value.

P M is the 2D-GC modulation period;

2 FWHH a is the second dimension peak width of the peak (a) at half height; and

2FWHH b is the second dimension peak width of the peak (b) at half height.

It follows from Equation 2 that two defined analytical targets being well separated from each other during the 2D-GC chromatographic process will have a relatively large s 2D value, whereas two defined analytical targets being very close to each other will be characterized by a relatively small Rs 2D value. Hence, defined analytical targets having neighbouring peaks (for example, peaks recorded with a retention time within +/- 30s) with a mutual Rs 2D value of 1 or above are well separated. In other words, the analytical process can be considered as maximal for this given defined analytical target.

Conversely, defined analytical targets having neighbouring peaks with mutual s 2D values below 1 are not to be well separated. Considering a poorly separated defined analytical target, the separation performance of the analytical process for this target is determined by the value of its mutual Rs 2D value and the number of neighbouring peaks with a mutual Rs 2D value below 1. In other words, the resolution of the analytical process depends on the number of peaks that are present within a cluster of dimension Rs 2D < 1. Illustrative examples of Rs 2D values, related to target separation cases, are given in Example 3. For the purpose of the present invention, defined analytical targets having no neighbouring peak with a mutual Rs 2D value smaller than 1 are defined as singletons (S); a defined analytical target having one neighbouring peak having a mutual Rs 2D value smaller than 1 is considered to belong to a single cluster (C); and a defined analytical target having several neighbouring peaks having mutual Rs 2D values less than 1 are considered to belong to several clusters. The clustering procedure and cluster counting, according to the present invention, are explained more fully in Table 8. In this Table, 17 defined analytical targets were found to have a Rs 2D value smaller than 1 and 17 defined analytical targets were found to belong to 11 clusters, whereas 78 defined analytical targets were found to belong to Singletons.

Furthermore, the present invention defines a 2D separation efficiency parameter (SE 2D ) for a 2D- GC set-up (Equation 3, below), as the percentage of the total number of defined analytical targets being resolved by a 2D-GC chromatographic process, considering than a defined analytical target belonging to a singleton has a contribution of 1, and a defined analytical target belonging to only one cluster has a contribution to SE 2D of its mutual Rs 2D value, whereas a defined analytical target belonging to several clusters has contributes to SE 2D in an amount equivalent to the product of all of its mutual Rs 2D values, as set forth in the equation below.

Equation 3 where

n is the number of Singletons;

m is the number of defined analytical targets belonging to clusters; o is the number of clusters including a given defined analytical target; and

Rs 2D y is the s 2D value for a defined analytical target / ' in a given cluster j.

The applicant has found that a method conforming to the present invention, the Separation Efficiency (SE 2D ) of a two-dimensional comprehensive gas chromatography set-up must be higher than 94%, and particularly higher than 95%. In other words, the percentage of unresolved defined analytical targets ( n SE 2D ), as defined by equation (2), must be lower than 6%, and particularly lower than 5%. n SE 2D = 100 - SE 2D Equation 4

Any combination of stationary phases employed in a 2D GC set up that provides a (SE 2D ) value above this threshold is a preferred combination in pursuance of the present invention.

Furthermore, in a more particular embodiment of the invention, the peak capacity (n Cj 2D ) of a 2D- GC set-up , as defined in more details here under, is higher than 4000, more particularly higher than 4500.

The peak capacity is defined by equation 5 (see L.M. Blumberg et al., J. Chromatogr. A 1188 (2008) 2-16. L.M. Blumberg et al., J. Sep. Sci. 31 (2008) 3352-3357, which is hereby incorporated by reference) Equation 5

where

obs„

n C; 2D is the observed 2D peak capacity for a given 2D-GC set- s l n c is the observed first dimension peak capacity; and

s ,2 n c the observed second dimension peak capacity. obs.l

n c is given by equation 6 (see Klee et al. J. Chrom. A 1383, 151-9 (2015)).

t Equation 6

( I M + l) x P M where

lt last s the first dimension retention time of the last eluting compound; l t first is the first dimension retention time of the first eluting compound;

P M is the modulation period; and

M r is the number of the average number of time each peak is sampled by the modulator, as described hereunder, rounded to the upper value. A similar equation is used for obs,2 n c , with subscript index 2, instead of 1.

Finally, the applicant has used equation 7 for obs,2 n c , based on the method proposed by Lan et al. Anal. Chem. 71 (1999) 709-714, which is hereby incorporated by reference, where a and b are fitting parameters for a given 2D-GC set-up. These parameters are listed in Table 10. Equation 7

\fa fa

As state herein above, the methodology according to the present invention can be employed to resolve any defined analytical targets from a complex mixture. However, in a particular embodiment of the present invention, the defined analytical targets are a group of 95 known or suspected allergens, as set forth in Table 1 below.

Table 1:

Extended list of potentially allergenic organic

CAS#

substances and other regulated substances

Acetyl Cedrene (main isomer) 32388-55-9

Alpha Isomethylionone 127-51-5

Amyl Cinnamic Alcohol (E) 101-85-9

Amyl Cinnamic Aldehyde (E) 122-40-7

Amyl Salicylate (ISO-) 87-20-7

Amyl Salicylate (N-) 2050-08-0

Anethole Trans (E) 4180-23-8

Anisyl Alcohol 105-13-5

Benzaldehyde 100-52-7

Benzyl Alcohol 100-51-6

Benzyl Benzoate 120-51-4

Benzyl Cinnamate (E) 103-41-3 Benzyl Cyanide 140-29-4

Benzyl Salicylate 118-58-1

Camphor 76-22-2

Carvone 99-49-0

Caryophyllene Beta 87-44-5

Cinnamic Alcohol (E) 104-54-1

Cinnamic Aldehyde (E) 104-55-2

Citronellol 106-22-9

Coumarin 91-64-5

Hydroxyisohexyl 3-cyclohexene carboxaldehyde

31906-04-4 (Cyclohexal / Lyral major)

Hydroxyisohexyl 3-cyclohexene carboxaldehyde

51414-25-6 (Cyclohexal / Lyral minor)

Damascenone Beta 23696-85-7

Damascone Alpha (E) 24720-09-0

Damascone Alpha (Z) 23726-94-5

Damascone Beta (E) 23726-91-2

Damascone Beta (Z) 23726-92-3

Damascone Delta cis/trans 71048-83-4

Damascone Delta trans/cis n/a

Damascone Delta trans/trans 71048-82-3

Di Iso-Butyl Phthalate 84-69-5

Di isopentyl phthalate 605-50-5

Di Isopropyl Phthalate 605-45-8

Di n-Butyl Phthalate 84-74-2

Di n-pentyl phthalate 131-18-0

Dicyclohexyl phthalate 84-61-7

Diethyl Hexyl Phthalate 117-81-7

Diethyl Phthalate 84-66-2

Dimethyl Phthalate 131-11-3

Dimethyl Benzyl Carbinyl Acetate 151-05-3

Ebanol 1 67801-20-1

Ebanol 2 67801-20-1

Estragol 140-67-0

Eugenol 97-53-0

Eugenyl acetate 93-28-7

Farnesol (E)(E) 106-28-5 Farnesol (Z)(E) 3790-71-4

Farnesol (E)(Z) 3879-60-5

Farnesol (Z)(Z) 16106-95-9

Galaxolide (Cis) 252933-49-6

Galaxolide (Trans) 252933-48-5

Geranial 141-27-5

Geraniol 106-24-1

Geranyl Acetate 105-87-3

Hexadecanolide 109-29-5

Hexyl Cinnamic Aldehyde (E) 101-86-0

Hydroxycitronellal 107-75-5

Iso E Super Alpha 68155-66-8

Iso E Super Beta 54464-57-2

Iso E Super Gamma 68155-67-9

Iso E Super minor 54464-59-4

Isoeugenol (E) 5932-68-3

Isoeugenol (Z) 5912-86-7

Isoeugenyl Acetate 93-29-8

Lilial 80-54-6

Limonene 5989-27-5

Linalool 78-70-6

Linalyl Acetate 115-95-7

Majantol 103694-68-4

Menthol 1490-04-6

Methoxycoumarin-7 531-59-9

Methyl Eugenol 93-15-2

Methyl Heptine Carbonate 111-12-6

Methyl Octine Carbonate 111-80-8

Methyl Salicylate 119-36-8

Neral 106-26-3 n-pentyl isopentyl phthalate 84777-06-0

Phenyl Acetaldehyde 122-78-1

Pinene Alpha 80-56-8

Pinene Beta 127-91-3

Propylidene Phthalide 3- (E) 56014-72-3

Propylidene Phthalide 3- (Z) 94704-89-9 Salicylaldehyde 90-02-8

Santalol Alpha 115-71-9

Santalol Beta 77-42-9

Sclareol 515-03-7

Terpinene Alpha 99-86-5

Terpineol Alpha 98-55-5

Terpineol Beta cis 7299-41-4

Terpineol Beta trans 7299-40-3

Terpineol Delta 7299-42-5

Terpineol Gamma 586-81-2

Terpinolene 586-62-9

Vanillin 121-33-5

In a method according to the present disclosure, a complex mixture of perfume ingredients containing one or more of the known or suspected allergens recited in Table 1 may be separated in a comprehensive two-dimensional gas chromatography set-up, equipped with a dual-stage cryogenic modulator. A first separation is obtained on the first column and portions of the eluted, partly separated substances from this first column are accumulated and concentrated by a thermal modulator, before being re-injected into the second, much shorter column, where a second, much faster separation is achieved. The differences in separation times allows multiple second separations to be completed over the duration of the first separation. The concentration- release step in the thermal modulator is determined by the duration of separation in the second column. The set-up is furthermore completed by one detector, the function of which is to measure a signal directly related to the concentration of defined analytical targets in the eluted streams coming out of the secondary column. The output of such a 2D-GC set-up is a two- dimensional plot combining the information in a visual way. The elution sequence from the first column is reported on an x-axis (first dimension) of the plot, whereas the several elution sequences from the second column are reported on y-axes (second dimension), as show in Figure 1 (From T. Dutriez, "GCxGC: a disruptive technique" in Gas Chromatography and 2D-GC chromatography for petroleum industry. F. Bertoncini, M. Courtiade-Tholance, D. Thiebaut (Editors) Editions Technip. 2013, p. 46).

Operating comprehensive gas chromatography equipment requires that a number parameters of the instrumental set-up are controlled. As will be apparent to a person skilled in the art, such parameters include the operating temperature and temperature program, injector split ratio, modulation period and column length and inner diameter.

In an embodiment of the invention, the temperature of the first column (main oven) is from subzero °C temperature to about 450 °C, more particularly from about 30 °C to about 350 °C. This temperature may be constant, but is generally increased at a given rate, starting from a temperature TO and ending at a temperature Tn. The rate of heating is typically from about 0. 1 °C/min to about 25 °C/min, more particularly from about 1 °C/min to 15 °C/min. The temperature program may also include one or more insothermal plateau at one or different pre-set temperature(s) and different heating rates may be combined within a given analytical process. The temperature of the second column (secondary oven) may be identical to that of the first column or different. In an embodiment of the invention, the temperature of the secondary oven is from about 5 °C to about 35 °C, more particularly from about 10 to about 30 °C higher than that of the main oven.

The injector split ratio, i.e. the ratio of the injected sample which effectively transferred to the first column, may be from about 1:1 to 1:150, more particularly from 1:75 to 1:125.

The modulation period, i.e. the time between two thermally-induced injections in the second column of the eluate coming out of the first column, is from about 2 to about 10 seconds, more particularly between 4 and 8 seconds. During the modulation period, the eluate coming out from the first column is cool-trapped or absorbed on a microporous material. The modulator may operate this action several time during the time a peak is eluting from the first column. This is expressed by the term M r in Equation 2.

In an embodiment of the invention, the eluate of the first column is cool-trapped at a temperature from about -150 °C to about to -70 °C, more particularly from -120 °C to -80 °C.

The clustering analysis methodology described herein provides that once a combination of stationary phases are found that satisfy the SE 2D threshold value described hereinabove, a 2D-GC set-up containing that stationary phase combination will be able to resolve any of the 95 known or suspected allergens in any complex mixture of perfume ingredients.

The applicant surprisingly found that the desired Separation Efficiency (SE 2D ) disclosed hereinabove of at least 94% and more particularly at least 95% can be achieved with a selection of stationary phases wherein the first stationary phase has an intermediate polarity, and the second stationary phase that is relatively polar compared with the first stationary phase. Such a selection of stationary phases is a preferred means to improve the resolution of the up to 95 known or suspected allergens set forth in Table 1. Accordingly,in a particular embodiment of the invention there is provided a method of resolving defined known or suspected allergens contained in a complex mixture of perfume ingredients, said method comprising the steps of analyzing the complex mixture using two-dimensional gas chromatography, wherein the first stationary phase has an intermediate polarity, and the second stationary phase is relatively polar compared with the first stationary phase. In a more particular embodiment the first stationary phase of intermediate polarity is an arylene- modified diphenyl-dimethyl siloxane copolymer stationary phase, more particularly having about 35% diphenylsiloxane moieties and about 65% dimethylsiloxane and arylene dimethyl siloxane moieties (Formula 1); and the second stationary phase that is relatively polar compared with the first is a (polyethylene-glycol) wax stationary phase. This combination of stationary phases provided good 2D separation efficiency for complex mixtures containing defined analytical targets of Table 1.

It was not expected that the first arylene-modified stationary phase would be useful because it is generally considered that arylene-modified stationary phases are highly specific to halogenated analytes, such as polychlorinated biphenyls and arochlor pesticides, and organophosphorous compounds.

Formula 1

Alternative arylene-modified diphenyl- and arylene dimethyl siloxane copolymer stationary phases with different ratios of diphenylsiloxane and arylene dimethyl siloxane moieties (See Formula 2) such as Agilent DB-5ms and Phenomenex ZEB ON ZB-5ms (with X% = about 5% diphenylsiloxane and Y% = about 95% arylene dimethyl siloxane) are also useful as intermediate polarity first stationary phases

Formula 2

Other stationary phases can be employed as intermediate polarity first stationary phases, for example those having unmodified poly(diphenylsiloxane-co-dimethylsiloxane) with about 35% diphenylsiloxane moieties, but no arylene or phenylene groups in the backbone are similar to the herein above mentioned arylene-modified analogues. Examples of such intermediate polar stationary phases are commercially available under various brands and Trademarks, such as Agilent J&W VF-35ms , Restek Rtx ® -35, Restek Rtx ® -35ms, Restek Rxi ® -35Sil MS, Supelco SPB-35, Alltech™ Heliflex™ AT™ -35, Supelco Sup-Herb, VB-35 - ValcoBond ® , SGC BPX-34, Phenomenex ZB- 35 HT, and the like.

In further embodiments of the invention, the intermediate polarity first stationary phase is an arylene-modified stationary phase comprising from about 20 to about 60 wt% diphenylsiloxane moieties and about 40 to about 80 wt% arylene dimethyl siloxane moieties, more particularly from about 30 to about 40 wt% diphenylsiloxane groups and from about 60 to 70 wt% arylene dimethyl siloxane moieties, and still more particularly from about 33 to about 38 wt% diphenylsiloxane moieties and from about 62 to about 67 wt% arylene dimethyl siloxane moieties, wherein the weight percentage (wt%) is relative to the total weight of the polymer. Examples of such intermediate polarity stationary phases are Agilent J&W VF-35ms, and Agilent DB-35ms, and the like.

In a more particular embodiment, the intermediate polarity first stationary phase is Agilent J&W VF-35ms. In an embodiment of the invention, the polar stationary phase comprises a poly(ethylene oxide) polymer. Examples of such polar stationary phases are commercially available under various brands and Trademarks, such as estek Rtx ® -Wax, Restek Stabilwax, Agilent DB Wax, Agilent CB

Wax SUPELCOWAX 10, SUPEROX II, SGE BP-20, 007-CW, Carbowax, Phenomenex® ZB-WAX, Phenomenex ® ZB-WAX plus, and the like.

In a particular embodiment, the polar stationary phase is Restek Stabil-Wax ® .

In an embodiment of the invention, the length of the column containing the first stationary phase is between 30 and 70 m, more particularly between 50 and 60 m.

In an embodiment of the invention and the diameter of the column containing the first stationary phase is between 0.15 and 0.32 mm, more particularly between 0.2 and 0.25 mm.

In an embodiment of the invention, the thickness of the first stationary phase is between 0.05 and 1 micrometers, more particularly between 0.25 and 0.50 micrometers.

In an embodiment of the invention, the length of the column containing the second stationary phase is between 0.5 and 3 m, more particularly between 0.8 and 2 m. In an embodiment of the invention the diameter of the column containing the second stationary phase is between 0.05 and 0.25 mm, more particularly between 0.1 and 0.2 mm.

In an embodiment of the invention, the thickness of the second stationary phase is between 0.05 and 1 micrometers, more particularly between 0.1 and 0.5 micrometers.

Once separated according to the present invention, the analytical targets are detected by using a flame ionization detector, a mass spectrometry detector or any detector having a suitable detection sensitivity and, for example, capable of transforming the molecular flow coming out of the second column into an electrical signal that is proportional to the concentration of the analytical target in the flow. Additionally, a mass spectrometry detector is use to further identify the chemical nature of the analyte by breaking the molecules into electrical charged fragments, the mass of which can be, for example, quantified as a function of the time of flight of each fragment between the locus of ionization and a detection device. Ionization occurs, for example, by exposure of the analyte to an electrical field providing a ionization energy of from 10 to 100 eV (electron-volt), more particularly from 50 to 80 eV. More details about gas chromatography / mass spectrometry coupling may be found in the book of S. Bouchonnet, "Introduction to GC-MS Coupling", C C Press, 2013, which is hereby incorporated by reference.

The method according to the present invention can be applied in a number of situations where a large number of defined analytical targets must be separated in view of their identification and/or quantification. Such complex mixtures include, but are not limited to perfumes, fragrances, flavours, petroleum hydrocarbons, polycyclic aromatic compounds, polychlorobiphenyls, pesticides, herbicides, metabolites, and the like.

Analytical methods described herein are particularly useful in helping perfumers to prepare compositions that are free or substantially free of any known or suspected allergens set forth in Table 1 hereinabove.

For perfume compositions that are intended to be employed in consumer products that are rinse- off products, such as personal care or cosmetic rinse-off products, it is preferred that if any of the known or suspected allergens are present, then each allergen should be present in amounts of 100 ppm or lower in a product. For products that are leave-on, the level of individual allergens preferably should not exceed 10 ppm in a product. Perfume compositions intended for rinse-off applications are considered to be substantially free of any known or suspected allergens if levels of individual allergens do not exceed 100 ppm in a product. Perfume compositions intended for leave-on applications are considered to be substantially free of any known or suspected allergens if levels of individual allergens do not exceed 10 ppm in a product. FIGURES

Figure 1: Representation of neighbouring peaks on a 2D GC plot;

Figure 2: Separation of Damascenone Beta and and Damascone Alpha (VF35 x Wax; Rs 2D =

0.74). These two analytical targets are clustered, according to this invention.

Figure 3: Separation of Geranyl Acetate and and Damascone Delta trans/trans (Rtx-5Sil x Wax;

Rs 2D =0.93). These two analytical targets are clustered, according to this invention.

Figure 4: Separation of Cyclohexal / Lyral minor and Cyclohexal / Lyral major (VF35 x Wax; Rs 2D

= 1.23). These two analytical targets are Singletons, according to this invention. Figure 5: Separation of Carvone and Geranial (VF35 x Wax; s 2D =1.35). These two analytical targets are Singletons, according to this invention.

EXAMPLES

Example 1: two-dimensional gas chromatographic procedure The 95 ingredients reported in Table 1 (see description herein above) were dissolved in METHYL TERT-BUTYL ETHER at a level of 250 ppm (0.0250% by weight) each. In cases an ingredient was a mixture of isomers, the amount was adapted in such a way that the most abundant isomer was at a level of 250 ppm in the solution.

All GCxGC experiments were carried out using with a Pegasus 4D GCxGC-TOFMS from LECO (St. Joseph, Ml, USA), consisting of a 7890B GC from (Agilent Technologies, USA), a LN2 cooled thermal modulator from LECO and a Pegasus HT TOFMS from LECO. The MS part was operated in an El mode at -70 eV, with an acquisition frequency set at 150 Hz in a mass ranging from 35 to 350 g/mol and with a multiple-plate voltage set at -1450 V. The GC transfer line was set at 245 °C and consisted of the secondary column. ChromaTOF (LECO) was used for controlling the 2D-GC set-up, for data acquisition and for data processing. Injections of the mixture of defined analytical targets were performed with a split injector with an injection temperature at 250 °C, a split ratio at 1:100 and an injection volume of 0.5 μί. Carrier gas (Helium) was delivered at a constant flow (1.3 mL/min). For comparison purpose, the same first column geometry was used for all 2D-GC set-ups investigated (60 m χ 0.25 mm ID, 0.25 μιτι film thickness). The reference length of the secondary column was set at 1 m (150 mm ID, 0.15 μιτι film thickness) and was possibly extended to 2 m in case of available 2D space with reference comparison parameters. Connections between the primary and the two secondary columns were done by a SilTite ® μ-Union (SGE Ringwood, Victoria, Australia). The reference 2D modulation period was set at 5 s with a hot pulse at 1.2 s (+15 °C versus the secondary column) and 2D modulation period was possibly extended to 7 s in case of wrap-around in secondary dimension with the reference comparison parameters.

A GC program-temperature ramp was implemented from 50 °C (1 min) to 245 °C when the 2D-GC set-up contains a Wax column and 300 °C when not (for several minutes depending of each 2D-GC set-up) at 2 °C/min (see Table 2). A reference temperature offset for the secondary column was set at +15 °C versus the main oven and was possibly extended to +25 °C m in case of wrap-around in secondary dimension with reference comparison parameters. Secondary dimension retention times were corrected with an offset from -0.5 s to -1.0 s in order to maximize the available 2D space. The exact set of parameters for each combination of stationary phases are reported in Table 2.

Table 2: Specific operating conditions for each 2D-GC set-up

Examples 2 to 6: Separation of defined analytical targets

The result of the two-dimensional gas chromatographic separation of the 95 allergens are reported in Tables 3 to 7 are the experimental data, including retention times in both first (\r) and second ( 2 tr) dimensions, width of the peak at half height in the second dimension ( 2 width), and the resolution between neighboring peaks (Rs 2D , from the first closest neighbouring peak to the fifth closest neighbouring peak).

Legend of Ta bles 3 to 7:

hr = First Dimension Time (s)

2tr = Second Dimension Time (s)

2 Width = Full Width at Half Height on secondary dimension

Rs 2D 1= Rs2D with the first neighbour

Rs 2D 2 = Rs2D with the second neighbour

Rs 2D 3 = Rs2D with the third neighbour Rs 2D 4 = Rs2D with the fourth neighbor

Rs 2D 5 = Rs2D with the fifth neighbour

TC SE 2D = Total contribution to SE2D. This total contribution is the sum of the Rs 2D for the corresponding target. Table 8 shows an example of how the ingredients are clustered, based on their Rs 2D and SE 2D values. The stationary phase combination was the same as in Table 3. The targets having neighbours with Rs 2D larger than 1 are singleton and therefore not reported in Table 7. As apparent from the table, TERPINEOL BETA TRANS and TERPINEOL DELTA have, for example, a mutual of 0.78, which is smaller than 1, and therefore belong to the same cluster CI. TERPINEOL DELTA has an additional neighbour peak width a of 1.58, which is larger than 1 and therefore means that this peak is sufficiently apart from TERPINEOL DELTA not to be in a cluster with the latter. (Note that Table 2 shows that this third target is MENTHOL).

Table 9 shows a comprehensive list of clustered targets, meaning all peaks having at least one neighbouring peak with Rs 2D smaller than 1. Table 10 summarizes all results from Tables 3 to 7 with the values of and parameters in Equations 1, 2, 5, 6 and 7.

Table 3: Experimental data for Rtx5 x Wax stationary phase combination (Example 2)

List of targets hr 2 tr 2 Width Rs 2D 1 Rs 2D 2 Rs 2D 2 Rs 2D Rs 2D 5 TC SE 2D

Acetyl Cedrene (main isomer) 4235 0.633 0.036966 7.155109 1

Alpha Isomethylionone 3227 0.514 0.035604 1

Amyl Cinnamic Alcohol (E) 3955 1.656 0.070874 4.178726 5.075817 5.137754 1

Amyl Cinnamic Aldehyde (E) 3829 0.923 0.047709 1.364748 1

Amyl Salicylate (ISO-) 3444 0.738 0.038064 1.047318 1

Amyl Salicylate (N-) 3584 0.777 0.039837 7.515063 1

Anethole Trans (E) 2499 0.963 0.053992 2.972017 12.76782 1

Anisyl Alcohol 2478 4.837 0.18442 10.88749 12.76782 1

Benzaldehyde 1148 1.359 0.070947 1

Benzyl Alcohol 1435 4.467 0.17169 16.15586 1

Benzyl Benzoate 4228 1.623 0.071624 7.155109 1

Benzyl Cinnamate (E) 5187 2.104 0.083973 6.511547 1

Benzyl Cyanide 1869 2.943 0.12699 1

Benzyl Salicylate 4543 1.728 0.071789 1

Camphor 1925 0.586 0.044176 2.23663 1

Carvone 2331 0.85 0.04671 2.379768 4.297913 1

Caryophyllene Beta 3038 0.303 0.031179 1

Cinnamic Alcohol (E) 2576 4.302 0.16619 1

Cinnamic Aldehyde (E) 2443 2.19 0.097562 8.205283 1

Citronellol 2247 0.949 0.047874 1

Coumarin 3087 3.702 0.15304 12.86211 1

Damascenone Beta 2870 0.646 0.041526 0.900152 1.289077 1.494049 1.632791 0.9001524

Damascone Alpha (E) 2912 0.567 0.039962 0.843133 1.200603 4.354721 16.06587 0.84313277

Damascone Alpha (Z) 2772 0.494 0.032495 11.03334 1

Damascone Beta (E) 2982 0.58 0.037195 6.781579 11.11522 1

Damascone Beta (Z) 2884 0.507 0.036201 1.036743 1.039212 1.200603 1.494049 1

Damascone Delta cis/trans 2891 0.6 0.036428 0.843133 0.900152 1.036743 0.75894799

Damascone Delta trans/cis 2688 0.487 0.033275 1

Damascone Delta trans/trans 2842 0.567 0.03833 0.93155 1.289077 0.9315502

Di Iso-Butyl Phthalate 4501 0.969 0.048177 1

Di isopentyl phthalate 5082 0.956 0.047532 1

Di Isopropyl Phthalate 3836 1.095 0.052944 1.364748 3.041261 5.054776 1

Di n-Butyl Phthalate 4781 1.068 0.050811 1

Di n-pentyl phthalate 5306 1.048 0.050069 1

Dicyclohexyl phthalate 6195 3.279 0.13412 1

Diethyl Hexyl Phthalate 6251 1.781 0.081122 1

Diethyl Phthalate 3626 1.517 0.068273 1

Dimethyl Benzyl Carbinyl Acetate 2618 0.692 0.050032 1

Dimethyl Phthalate 3122 2.19 0.091771 1.526838 9.391394 9.738884 1

Ebanol 1 3108 0.6 0.036457 1.108452 9.738884 10.95377 12.86211 1

Ebanol 2 3136 0.639 0.037954 1.108452 9.391394 10.62555 1

Estragol 2135 0.81 0.0464 0.515836 0.542744 0.788273 3.333814 0.22069028

Eugenol 2758 2.223 0.090546 11.03334 1

Eugenyl acetate 3367 1.438 0.064632 1

Farnesol (E)(E) 4053 0.89 0.045083 1.892172 12.56978 1

Farnesol (E)(Z) 3983 0.86 0.053156 0 2.381348 5.075817 0

Farnesol (Z)(E) 3983 0.86 0.053156 0 2.295438 5.137754 0

Farnesol (Z)(Z) 3892 0.85 0.041714 3.008755 3.086871 3.306978 4.862365 5.076328 1

Galaxolide (Cis) 4459 0.613 0.039151 0.264398 0.26439839

Galaxolide (Trans) 4466 0.619 0.038465 0.264398 0.26439839

Geranial 2422 0.738 0.041848 8.205283 1

Geraniol 2345 1.154 0.05591 2.379768 6.469175 1

Geranyl Acetate 2856 0.494 0.03541 0.93155 1.039212 1.632791 0.9315502

Hexadecanolide 4725 0.593 0.036262 1

Hexyl Cinnamic Aldehyde (E) 4151 0.89 0.045452 1

Hydroxycitronellal 2492 1.405 0.063091 2.972017 10.88749 1

Hydroxyisohexyl 3-cyclohexene carboxaldehyde

(Cyclohexal / Lyral major) 3892 1.53 0.067972 1.030023 4.862365 7.402963 7.452571 7.637425 1

Hydroxyisohexyl 3-cyclohexene carboxaldehyde

(Cyclohexal / Lyral minor) 3864 1.524 0.064631 1.030023 3.041261 5.076328 7.6884 7.776542 1

Iso E Super Alpha 3997 0.606 0.035899 2.295438 2.381348 1

Iso E Super Beta 3885 0.547 0.035541 0.772059 1.053415 3.086871 7.452571 7.6884 0.77205882

Iso E Super Gamma 3913 0.567 0.034613 1.053415 3.008755 4.277514 7.402963 1

Iso E Super minor 3864 0.547 0.033905 0.772059 3.306978 5.054776 7.637425 7.776542 0.77205882

Isoeugenol (E) 3122 2.573 0.10497 1.526838 10.62555 10.95377 1

Isoeugenol (Z) 2961 2.349 0.087931 7.175595 11.11522 1

Isoeugenyl Acetate 3689 1.642 0.072461 1

Lilial 3416 0.758 0.043279 1.047318 1

Limonene 1421 0.256 0.032844 16.15586 1

Linalool 1715 0.718 0.042539 1

Linalyl Acetate 2345 0.408 0.034534 4.297913 6.469175 1

Majantol 2996 1.477 0.066846 6.781579 1

Menthol 2051 0.758 0.045037 1.581179 1

Methoxycoumarin-7 4081 4.236 0.1644 11.3582 12.56978 1

Methyl Eugenol 2940 1.068 0.052903 4.354721 7.175595 14.11996 1

Methyl Heptine Carbonate 2135 0.72 0.043148 0.788273 1.108792 1.261058 4.13508 0.78827261

Methyl Octine Carbonate 2541 0.679 0.041633 1

Methyl Salicylate 2114 1.233 0.055896 2.823862 3.333814 4.13508 1

Neral 2296 0.712 0.039618 1 n-pentyl isopentyl phthalate 5194 1.002 0.048866 6.511547 1

Phenyl Acetaldehyde 1477 1.491 0.066865 1.510067 1

Pinene Alpha 1043 0.164 0.033474 1

Pinene Beta 1218 0.21 0.038099 1

Propylidene Phthalide 3- (E) 3570 1.979 0.085905 7.515063 1

Propylidene Phthalide 3- (Z) 3731 2.263 0.093138 1

Salicylaldehyde 1484 1.761 0.075452 1.510067 1

Santalol Alpha 3934 1.022 0.050207 4.178726 4.277514 1

Santalol Beta 4067 1.114 0.051404 1.892172 11.3582 1

Sclareol 5516 1.689 0.072529 1

Terpinene Alpha 1372 0.243 0.030979 1

Terpineol Alpha 2128 0.864 0.048338 0.515836 0.823545 1.261058 2.823862 0.42481459

Terpineol Beta cis 1932 0.831 0.042312 2.23663 1

Terpineol Beta trans 2009 0.956 0.046408 0.783489 0.78348909

Terpineol Delta 2023 0.89 0.041224 0.783489 1.581179 0.78348909

Terpineol Gamma 2149 0.83 0.0447 0.542744 0.823545 1.108792 0.44697387

Terpinolene 1659 0.289 0.029896 1

Vanillin 2926 6.619 0.25564 14.11996 16.06587 1

Table 4: Experimental data for Rtx5 x Rxl7 stationary phase combination (Example 3)

List of targets hr 2 tr 2 Width Rs 2D 1 Rs 2D 2 Rs 2D 2 Rs 2D 4 Rs 2D 5 TC SE 2D

Acetyl Cedrene (main isomer) 4290 2.085 0.078985 4.21 1.00

Alpha Isomethylionone 3280 1.655 0.070744 1.00

Amyl Cinnamic Alcohol (E) 4005 2.2 0.07523 2.11 3.33 3.40 1.00

Amyl Cinnamic Aldehyde (E) 3880 2.19 0.076798 1.09 1.00

Amyl Salicylate (ISO-) 3495 1.85 0.066083 1.68 1.00

Amyl Salicylate (N-) 3640 1.89 0.064649 5.29 1.00

Anethole Trans (E) 2555 2.07 0.067802 1.68 3.55 1.00

Anisyl Alcohol 2535 2.735 0.084998 3.55 4.79 1.00

Benzaldehyde 1190 1.96 0.083965 1.00

Benzyl Alcohol 1480 2.11 0.079133 5.01 1.00

Benzyl Benzoate 4280 3.005 0.093454 4.21 1.00

Benzyl Cinnamate (E) 5245 3.33 0.1021 3.87 1.00

Benzyl Cyanide 1925 2.84 0.089987 1.00

Benzyl Salicylate 4600 2.965 0.089558 1.00

Camphor 1980 1.845 0.10754 1.66 1.00

Carvone 2380 2.035 0.075333 2.14 2.97 4.15 1.00

Caryophyllene Beta 3095 1.415 0.067419 1.00

Cinnamic Alcohol (E) 2630 2.595 0.082422 1.00

Cinnamic Aldehyde (E) 2495 2.74 0.083831 5.26 1.00

Citronellol 2300 1.375 0.061069 1.00

Coumarin 3140 3.785 0.11183 10.56 1.00

Damascenone Beta 2925 1.885 0.07937 1.03 1.03 1.50 2.15 1.00

Damascone Alpha (E) 2965 1.795 0.07685 0.99 1.23 2.88 6.48 0.99

Damascone Alpha (Z) 2825 1.715 0.078681 2.59 1.00

Damascone Beta (E) 3040 1.835 0.078473 1.00 2.86 1.00

Damascone Beta (Z) 2940 1.777 0.038692 0.37 1.03 1.23 2.48 0.37

Damascone Delta cis/trans 2945 1.82 0.08277 0.37 0.99 1.03 6.31 0.37

Damascone Delta trans/cis 2740 1.655 0.077153 1.00

Damascone Delta trans/trans 2900 1.715 0.075344 1.20 1.50 1.00

Di Iso-Butyl Phthalate 4555 2.36 0.082806 1.00

Di isopentyl phthalate 5140 2.36 0.08633 1.00

Di Isopropyl Phthalate 3890 2.39 0.084574 1.09 1.51 2.83 1.00

Di n-Butyl Phthalate 4835 2.51 0.085801 1.00

Di n-pentyl phthalate 5355 2.485 0.082997 1.00

Dicyclohexyl phthalate 6255 3.825 0.11476 1.00

Diethyl Hexyl Phthalate 6300 2.37 0.081362 1.00

Diethyl Phthalate 3675 2.745 0.090351 1.00

Dimethyl Benzyl Carbinyl Acetate 2670 1.83 0.075734 1.00

Dimethyl Phthalate 3175 3.02 0.095451 2.92 7.80 7.86 1.00

Ebanol 1 3160 1.43 0.063834 5.37 7.86 10.56 1.00

Ebanol 2 3195 1.435 0.065157 5.26 7.80 1.00

Estragol 2190 1.865 0.06567 0.46 1.61 1.69 1.69 0.46

Eugenol 2815 2.215 0.075385 2.59 1.00

Eugenyl acetate 3420 2.58 0.084525 1.00

Farnesol (E)(E) 4110 1.7 0.062999 1.78 1.00

Farnesol (E)(Z) 4035 1.655 0.064011 0.00 1.73 3.40 0.00

Farnesol (Z)(E) 4035 1.66 0.066779 0.00 1.68 3.33 0.00

Farnesol (Z)(Z) 3970 1.691 0.054276 1.23 1.37 1.67 4.00 1.00

Galaxolide (Cis) 4515 2.22 0.083539 0.26 0.26

Galaxolide (Trans) 4520 2.235 0.082772 0.26 0.26

Geranial 2470 1.755 0.067246 5.26 1.00

Geraniol 2400 1.54 0.063025 1.50 2.97 1.00

Geranyl Acetate 2910 1.525 0.060094 1.20 2.15 2.48 1.00

Hexadecanolide 4785 2.145 0.078587 1.00

Hexyl Cinnamic Aldehyde (E) 4210 2.155 0.075698 1.00

Hydroxycitronellal 2545 1.785 0.071342 1.68 4.79 1.00

Hydroxyisohexyl 3-cyclohexene carboxaldehyde

(Cyclohexal / Lyral major) 3945 2.34 0.079505 1.23 2.32 2.62 2.79 4.00 1.00

Hydroxyisohexyl 3-cyclohexene carboxaldehyde

(Cyclohexal / Lyral minor) 3920 2.315 0.080616 1.23 1.51 2.24 2.50 1.00

Iso E Super Alpha 4050 1.93 0.07364 1.68 1.73 1.00

Iso E Super Beta 3945 1.88 0.076174 1.23 1.47 1.67 2.32 2.50 1.00

Iso E Super Gamma 3970 1.89 0.07261 1.02 1.23 1.23 2.62 1.00

Iso E Super minor 3915 1.89 0.069418 1.47 2.24 2.79 2.83 1.00

Isoeugenol (E) 3180 2.38 0.077226 2.92 5.26 5.37 1.00

Isoeugenol (Z) 3015 2.333 0.072664 1.01 2.86 1.00

Isoeugenyl Acetate 3740 2.69 0.08576 1.00

Lilial 3470 2.055 0.074164 1.68 1.00

Limonene 1475 1.055 0.08622 5.01 1.00

Linalool 1765 1.225 0.073398 1.00

Linalyl Acetate 2395 1.295 0.066895 1.50 4.15 1.00

Majantol 3050 2.005 0.07398 1.00 1.00

Menthol 2105 1.4 0.069163 1.77 1.00

Methoxycoumarin-7 4145 4.14 0.12153 8.68 1.00

Methyl Eugenol 2995 2.285 0.078575 1.01 2.88 4.32 1.00

Methyl Heptine Carbonate 2185 1.8 0.067148 0.46 1.25 1.44 1.79 0.46

Methyl Octine Carbonate 2595 1.77 0.064649 1.00

Methyl Salicylate 2170 2.09 0.072635 1.61 1.79 2.82 3.12 1.00

Neral 2355 1.71 0.069514 2.14 1.00 n-pentyl isopentyl phthalate 5250 2.416 0.083471 3.87 1.00

Phenyl Acetaldehyde 1525 2.22 0.08114 0.71 0.71

Pinene Alpha 1090 0.795 0.092236 1.00

Pinene Beta 1265 0.965 0.098099 1.00

Propylidene Phthalide 3- (E) 3625 2.925 0.090344 5.29 1.00

Propylidene Phthalide 3- (Z) 3785 3.175 0.096111 1.00

Salicylaldehyde 1535 2.115 0.079171 0.71 0.71

Santalol Alpha 3990 1.84 0.067159 1.02 1.37 2.11 1.00

Santalol Beta 4125 1.985 0.07445 1.78 8.68 1.00

Sclareol 5570 2.545 0.083208 1.00

Terpinene Alpha 1420 1.035 0.083167 1.00

Terpineol Alpha 2180 1.585 0.070044 0.98 1.25 1.69 2.82 0.98

Terpineol Beta cis 1985 1.46 0.075841 1.66 1.00

Terpineol Beta trans 2060 1.545 0.076965 0.76 0.76

Terpineol Delta 2075 1.585 0.077601 0.76 1.77 0.76

Terpineol Gamma 2200 1.58 0.07256 0.98 1.44 1.69 3.12 0.98

Terpinolene 1715 1.23 0.07357 1.00

Vanillin 2975 3.225 0.096758 4.32 6.31 6.48 1.00

Table 5: Experimental data for Wax x Rx5 stationary phase combination (Example 4)

List of targets hr 2 tr 2 Width Rs 2D 1 Rs 2D 2 Rs 2D 2 Rs 2D 4 Rs 2D 5 TC SE 2D

Acetyl Cedrene (main isomer) 4415 2.11 0.065 1.00

Alpha Isomethylionone 3310 2.08 0.064 9.11 1.00

Amyl Cinnamic Alcohol (E) 5185 0.915 0.037 0.76 3.84 0.76

Amyl Cinnamic Aldehyde (E) 4490 1.335 0.047 4.12 6.05 1.00

Amyl Salicylate (ISO-) 3880 1.545 0.050 1.34 5.19 7.74 1.00

Amyl Salicylate (N-) 4075 1.49 0.049 1.00

Anethole Trans (E) 3250 1.12 0.040 4.34 1.00

Anisyl Alcohol 4550 0.54 0.030 0.55 8.23 0.55

Benzaldehyde 2230 0.75 0.036 1.00

Benzyl Alcohol 3400 0.49 0.028 11.16 1.00

Benzyl Benzoate 5405 1.01 0.040 1.00

Benzyl Cinnamate (E) 6865 1.62 0.055 1.00

Benzyl Cyanide 3565 0.595 0.031 1.00

Benzyl Salicylate 5760 1.04 0.039 1.00

Camphor 2190 1.66 0.054 1.00

Carvone 2945 1.245 0.043 0.51 5.93 0.51

Caryophyllene Beta 2480 4.115 0.113 1.00

Cinnamic Alcohol (E) 4560 0.56 0.031 0.55 8.08 0.55

Cinnamic Aldehyde (E) 3895 0.73 0.033 7.17 7.74 12.28 1.00

Citronellol 3040 1.005 0.038 3.94 6.39 6.76 1.00

Coumarin 4985 0.665 0.033 3.52 1.00

Damascenone Beta 3220 1.595 0.052 1.56 4.34 1.00

Damascone Alpha (E) 3130 1.795 0.057 0.31 0.31

Damascone Alpha (Z) 2830 2.075 0.064 6.84 6.98 1.00

Damascone Beta (E) 3210 1.8 0.057 1.56 1.00

Damascone Beta (Z) 2975 2.03 0.064 5.17 5.93 1.00

Damascone Delta cis/trans 3135 1.77 0.050 0.31 0.31

Damascone Delta trans/cis 2735 2.1 0.065 6.55 7.20 7.85 1.00

Damascone Delta trans/trans 3050 1.825 0.057 1.54 3.09 6.76 1.00

Di Iso-Butyl Phthalate 5195 1.33 0.048 3.84 4.32 1.00

Di isopentyl phthalate 5700 1.49 0.052 12.72 1.00

Di Isopropyl Phthalate 4685 1.125 0.042 1.72 1.89 7.24 1.00

Di n-Butyl Phthalate 5550 1.295 0.047 1.00

Di n-pentyl phthalate 5980 1.675 0.055 1.00

Dicyclohexyl phthalate 5710 4.415 0.128 12.72 1.00

Diethyl Hexyl Phthalate 6905 4.105 0.126 1.00

Diethyl Phthalate 4775 0.92 0.037 4.78 10.79 1.00

Dimethyl Benzyl Carbinyl Acetate 3065 1.42 0.049 3.09 3.94 4.52 1.00

Dimethyl Phthalate 4595 0.74 0.034 1.00

Ebanol 1 3415 1.67 0.055 11.16 1.00

Ebanol 2 3520 1.56 0.052 1.00

Estragol 2735 1.215 0.041 0.95 2.01 6.55 0.95

Eugenol 4250 0.715 0.032 1.00

Eugenyl acetate 4490 0.9 0.036 2.11 4.12 1.00

Farnesol (E)(E) 4735 1.28 0.046 1.00 1.42 5.87 7.80 1.00

Farnesol (E)(Z) 4660 1.26 0.046 1.52 1.72 5.86 6.10 1.00

Farnesol (Z)(E) 4630 1.305 0.046 1.52 5.64 5.69 1.00

Farnesol (Z)(Z) 4530 1.307 0.043 8.08 8.23 1.00

Galaxolide (Cis) 4640 2.11 0.065 0.75 5.69 6.10 0.75

Galaxolide (Trans) 4655 2.085 0.065 0.75 5.64 5.86 7.24 0.75

Geranial 2940 1.295 0.045 0.51 0.51

Geraniol 3305 0.91 0.036 9.11 1.00

Geranyl Acetate 3020 1.76 0.056 1.54 3.48 6.39 1.00

Hexadecanolide 4765 2.5 0.078 6.58 7.80 10.79 1.00

Hexyl Cinnamic Aldehyde (E) 4750 1.43 0.050 1.42 4.78 6.58 7.12 1.00

Hydroxycitronellal 3600 0.84 0.036 1.00

Hydroxyisohexyl 3-cyclohexene carboxaldehyde

(Cyclohexal / Lyral major) 5040 0.975 0.039 1.47 1.00

Hydroxyisohexyl 3-cyclohexene carboxaldehyde

(Cyclohexal / Lyral minor) 5010 0.97 0.039 1.47 3.52 1.00

Iso E Super Alpha 4135 2.145 0.066 9.59 1.00

Iso E Super Beta 3940 2.29 0.074 1.47 1.00

Iso E Super Gamma 3995 2.25 0.069 1.00

Iso E Super minor 3910 2.29 0.067 1.47 5.19 5.51 12.28 1.00

Isoeugenol (E) 4730 0.695 0.032 5.80 5.87 7.12 1.00

Isoeugenol (Z) 4490 0.715 0.033 2.11 6.05 1.00

Isoeugenyl Acetate 4915 0.875 0.035 0.49 3.34 0.49

Lilial 3905 1.475 0.049 1.34 5.51 7.17 1.00

Limonene 1070 2.72 0.075 1.00

Linalool 2305 1.12 0.040 1.00

Linalyl Acetate 2340 2.02 0.062 1.00

Majantol 4140 0.905 0.036 9.59 1.00

Menthol 2620 1.25 0.044 1.82 5.32 1.00

Methoxycoumarin-7 6145 0.805 0.038 1.00

Methyl Eugenol 3815 1.01 0.038 1.00

Methyl Heptine Carbonate 2665 1.21 0.042 4.85 1.00

Methyl Octine Carbonate 3000 1.33 0.046 3.48 5.17 1.00

Methyl Salicylate 3090 0.95 0.036 4.52 1.00

Neral 2770 1.34 0.046 2.46 6.29 1.00 n-pentyl isopentyl phthalate 5830 1.545 0.054 1.00

Phenyl Acetaldehyde 2650 0.755 0.032 4.85 5.32 1.00

Pinene Alpha 605 2.595 0.075 1.00

Pinene Beta 805 2.745 0.078 1.00

Propylidene Phthalide 3- (E) 4925 0.88 0.036 0.49 3.21 0.49

Propylidene Phthalide 3- (Z) 5195 0.86 0.037 0.76 4.32 0.76

Salicylaldehyde 2770 0.72 0.032 3.94 6.29 1.00

Santalol Alpha 4715 1.255 0.045 1.00 1.89 5.80 1.00

Santalol Beta 4925 1.205 0.043 3.21 3.34 1.00

Sclareol 6695 2.195 0.070 1.00

Terpinene Alpha 1010 2.7 0.074 1.00

Terpineol Alpha 2820 1.14 0.042 0.50 6.98 0.50

Terpineol Beta cis 2590 1.135 0.040 1.82 1.00

Terpineol Beta trans 2765 1.075 0.039 1.52 2.01 2.46 3.94 7.85 1.00

Terpineol Delta 2735 1.115 0.042 0.95 1.52 7.20 0.95

Terpineol Gamma 2830 1.15 0.042 0.50 6.84 0.50

Terpinolene 1350 2.72 0.075 1.00

Vanillin 5260 0.515 0.030 1.00

Table 6: Experimental data for Rtx-17 x Wax stationary phase combination (Example 5)

List of targets hr 2 tr 2 Width Rs 2D 1 Rs 2D 2 Rs 2D 2 Rs 2D 4 Rs 2D 5 TC SE 2D

Acetyl Cedrene (main isomer) 4375 0.84 0.0424 1.98 1.00

Alpha Isomethylionone 3245 0.77 0.0409 1.00

Amyl Cinnamic Alcohol (E) 4215 1.89 0.0749 1.36 2.52 4.64 1.00

Amyl Cinnamic Aldehyde (E) 4085 1.09 0.0503 1.62 2.19 2.43 4.45 1.00

Amyl Salicylate (ISO-) 3550 1.01 0.0452 13.64 1.00

Amyl Salicylate (N-) 3710 1.04 0.0459 4.97 1.00

Anethole Trans (E) 2770 1.105 0.0469 1.81 1.00

Anisyl Alcohol 2985 3.8 0.1346 12.12 14.13 1.00

Benzaldehyde 1465 1.435 0.0580 1.00

Benzyl Alcohol 1775 4.275 0.1502 1.00

Benzyl Benzoate 4730 1.51 0.0614 1.00

Benzyl Cinnamate (E) 5730 3.085 0.1144 1.23 1.00

Benzyl Cyanide 2430 2.26 0.0858 8.05 1.00

Benzyl Salicylate 5010 1.66 0.0650 1.00

Camphor 2100 0.77 0.0426 4.08 1.00

Carvone 2580 1.01 0.0468 0.42 0.42

Caryophyllene Beta 2865 0.525 0.0325 2.14 2.71 1.00

Cinnamic Alcohol (E) 3030 3.635 0.1304 11.32 11.70 12.54 13.11 1.00

Cinnamic Aldehyde (E) 2940 1.865 0.0728 7.40 1.00

Citronellol 2210 1.52 0.0635 2.05 1.00

Coumarin 3815 2.455 0.0939 5.77 1.00

Damascenone Beta 3035 0.85 0.0438 0.70 1.88 1.96 12.54 0.70

Damascone Alpha (E) 3030 0.78 0.0404 0.70 2.32 2.60 13.11 0.70

Damascone Alpha (Z) 2845 0.695 0.0378 0.80 2.14 0.80

Damascone Beta (E) 3115 0.78 0.0409 1.00

Damascone Beta (Z) 2990 0.705 0.0372 2.84 14.13 1.00

Damascone Delta cis/trans 2925 0.795 0.0411 1.61 7.40 1.00

Damascone Delta trans/cis 2725 0.71 0.0388 1.51 1.00

Damascone Delta trans/trans 2830 0.725 0.0359 0.80 0.80

Di Iso-Butyl Phthalate 4815 1.09 0.0487 1.00

Di isopentyl phthalate 5365 1.28 0.0573 1.00

Di Isopropyl Phthalate 4200 1.155 0.0509 2.26 3.37 3.45 4.64 1.00

Di n-Butyl Phthalate 5135 1.155 0.0513 1.00

Di n-pentyl phthalate 5615 1.665 0.0686 1.00

Dicyclohexyl phthalate 7095 3.9 0.1302 1.00

Diethyl Hexyl Phthalate 6680 2.935 0.1212 1.00

Diethyl Phthalate 4105 1.4 0.0590 0.84 2.43 4.58 0.84

Dimethyl Benzyl Carbinyl Acetate 2780 0.9 0.0455 1.81 1.00

Dimethyl Phthalate 3700 1.765 0.0691 4.97 1.00

Ebanol 1 3005 1 0.0472 1.96 2.32 2.84 11.70 12.12 1.00

Ebanol 2 3050 1.055 0.0490 1.88 2.60 7.64 11.32 1.00

Estragol 2335 0.995 0.0440 1.16 1.00

Eugenol 3075 2.37 0.0878 7.64 1.00

Eugenyl acetate 3825 1.35 0.0568 5.77 1.00

Farnesol (E)(E) 4095 1.3 0.0563 0.84 1.62 3.14 3.80 0.84

Farnesol (E)(Z) 4020 1.31 0.0573 0.25 1.19 0.25

Farnesol (Z)(E) 4015 1.31 0.0573 0.25 1.06 4.36 0.25

Farnesol (Z)(Z) 3925 1.12 0.0477 3.24 1.00

Galaxolide (Cis) 4670 0.78 0.0410 0.49 0.49

Galaxolide (Trans) 4680 0.78 0.0416 0.49 0.49

Geranial 2580 0.96 0.0469 0.42 0.42

Geraniol 2390 1.68 0.0675 1.78 1.00

Geranyl Acetate 2895 0.73 0.0380 1.61 2.71 1.00

Hexadecanolide 4850 0.8 0.0418 10.54 1.00

Hexyl Cinnamic Aldehyde (E) 4380 1.07 0.0495 1.98 1.00

Hydroxycitronellal 2675 1.72 0.0688 1.00

Hydroxyisohexyl 3-cyclohexene carboxaldehyde

(Cyclohexal / Lyral major) 4205 1.66 0.0671 1.16 1.23 1.36 3.37 1.00

Hydroxyisohexyl 3-cyclohexene carboxaldehyde

(Cyclohexal / Lyral minor) 4180 1.65 0.0666 1.23 1.30 1.46 3.45 1.00

Iso E Super Alpha 4080 0.835 0.0414 2.19 3.80 4.58 6.52 1.00

Iso E Super Beta 3960 0.77 0.0414 1.23 1.25 1.00

Iso E Super Gamma 3985 0.795 0.0411 1.25 4.36 5.20 1.00

Iso E Super minor 3935 0.765 0.0392 1.23 3.24 1.00

Isoeugenol (E) 3485 2.575 0.0945 1.00

Isoeugenol (Z) 3310 2.375 0.0803 11.56 1.00

Isoeugenyl Acetate 4160 1.51 0.0615 1.30 1.00

Lilial 3640 0.93 0.0452 1.00

Limonene 1240 0.435 0.0368 1.00

Linalool 1630 1.215 0.0534 1.00

Linalyl Acetate 2265 0.675 0.0368 1.00

Majantol 3205 1.785 0.0707 1.00

Menthol 1995 1.22 0.0532 1.00

Methoxycoumarin-7 4865 2.71 0.1007 10.54 1.00

Methyl Eugenol 3315 1.1 0.0495 11.56 1.00

Methyl Heptine Carbonate 2345 0.88 0.0421 1.16 1.00

Methyl Octine Carbonate 2720 0.865 0.0429 1.51 1.00

Methyl Salicylate 2390 1.4 0.0556 1.78 1.00

Neral 2440 0.925 0.0444 8.05 1.00 n-pentyl isopentyl phthalate 5485 1.455 0.0625 1.00

Phenyl Acetaldehyde 1865 1.475 0.0626 1.00

Pinene Alpha 825 0.285 0.0310 1.00

Pinene Beta 1040 0.35 0.0346 1.00

Propylidene Phthalide 3- (E) 4070 1.77 0.0714 3.14 4.45 6.52 1.00

Propylidene Phthalide 3- (Z) 4290 1.895 0.0721 1.00

Salicylaldehyde 1815 1.84 0.0692 1.00

Santalol Alpha 4005 1.45 0.0595 1.06 1.19 5.20 1.00

Santalol Beta 4200 1.475 0.0603 1.16 1.46 2.26 2.52 1.00

Sclareol 5745 2.8 0.1114 1.23 1.00

Terpinene Alpha 1205 0.415 0.0362 1.00

Terpineol Alpha 2175 1.245 0.0536 0.98 0.98

Terpineol Beta cis 1940 1.24 0.0536 1.00

Terpineol Beta trans 2060 1.33 0.0530 1.58 1.00

Terpineol Delta 2090 1.255 0.0513 1.58 4.08 1.00

Terpineol Gamma 2195 1.235 0.0534 0.98 2.05 0.98

Terpinolene 1545 0.48 0.0348 1.00

Vanillin 3540 4.595 0.1610 13.64 1.00

Table 7: Experimental data for VF35-MS x Wax stationary phase combination (Exam

List of targets hr 2 tr 2 Width Rs 2D 1 Rs 2D 2 Rs 2D 2 Rs 2D Rs 2D 5 TC SE 2D

Acetyl Cedrene (main isomer) 4470 0.695 0.038827 2.21 1.00

Alpha Isomethylionone 3375 0.61 0.036351 11.16 1.00

Amyl Cinnamic Alcohol (E) 4280 1.675 0.061175 0.79 1.50 3.21 0.79

Amyl Cinnamic Aldehyde (E) 4150 0.94 0.045905 1.35 1.38 2.38 3.08 3.51 1.00

Amyl Salicylate (ISO-) 3665 0.825 0.040867 6.14 1.00

Amyl Salicylate (N-) 3825 0.85 0.042853 3.27 1.00

Anethole Trans (E) 2820 0.965 0.045055 2.35 4.06 1.00

Anisyl Alcohol 3000 3.624 0.13571 14.02 1.00

Benzaldehyde 1510 1.285 0.057839 1.00

Benzyl Alcohol 1820 3.984 0.142 1.00

Benzyl Benzoate 4745 1.38 0.059077 5.94 6.00 1.00

Benzyl Cinnamate (E) 5740 2.175 0.086254 1.00

Benzyl Cyanide 2435 2.15 0.084839 5.37 8.23 8.96 10.91 1.00

Benzyl Salicylate 5035 1.515 0.061639 1.00

Camphor 2200 0.62 0.040015 3.77 4.24 1.00

Carvone 2640 0.86 0.043668 1.35 1.00

Caryophyllene Beta 3050 0.38 0.029971 3.12 15.28 1.00

Cinnamic Alcohol (E) 3040 3.49 0.12971 13.39 13.92 15.28 1.00

Cinnamic Aldehyde (E) 2945 1.755 0.072103 8.73 1.00

Citronellol 2350 1.225 0.05472 1.00

Coumarin 3775 2.42 0.094431 1.00

Damascenone Beta 3125 0.7 0.039164 0.74 0.76 1.99 9.29 0.56

Damascone Alpha (E) 3130 0.63 0.037497 0.75 0.76 2.13 9.89 0.57

Damascone Alpha (Z) 2955 0.56 0.03537 8.73 1.00

Damascone Beta (E) 3220 0.63 0.037841 2.24 1.00

Damascone Beta (Z) 3095 0.57 0.036877 1.26 1.99 10.39 1.00

Damascone Delta cis/trans 3115 0.645 0.038025 0.74 0.75 1.26 9.74 0.56

Damascone Delta trans/cis 2845 0.565 0.036046 2.13 2.15 4.06 1.00

Damascone Delta trans/trans 3035 0.64 0.037202 1.15 3.12 13.39 1.00

Di Iso-Butyl Phthalate 4880 0.94 0.045613 1.00

Di isopentyl phthalate 5435 0.97 0.046779 1.00

Di Isopropyl Phthalate 4245 1.02 0.048296 1.53 3.16 3.34 1.00

Di n-Butyl Phthalate 5190 1.015 0.04802 1.00

Di n-pentyl phthalate 5675 1.2 0.05484 1.00

Dicyclohexyl phthalate 7010 3.125 0.14422 1.00

Diethyl Hexyl Phthalate 6585 1.64 0.060233 1.00

Diethyl Phthalate 4120 1.285 0.054237 0.71 1.68 1.70 3.08 5.56 0.71

Dimethyl Benzyl Carbinyl Acetate 2865 0.755 0.042792 2.13 1.00

Dimethyl Phthalate 3685 1.675 0.069177 6.14 1.00

Ebanol 1 3160 0.785 0.041446 2.13 1.00

Ebanol 2 3200 0.835 0.041854 2.24 1.00

Estragol 2410 0.84 0.04148 1.60 3.36 8.23 1.00

Eugenol 3120 2.135 0.082054 9.29 9.74 9.89 10.39 1.00

Eugenyl acetate 3830 1.255 0.054525 3.27 1.00

Farnesol (E)(E) 4215 1.075 0.0498 1.53 2.98 3.85 1.00

Farnesol (E)(Z) 4140 1.1 0.051734 0.29 1.03 1.38 1.68 2.45 0.29

Farnesol (Z)(E) 4135 1.08 0.050734 0.29 1.00 1.35 1.70 2.71 0.29

Farnesol (Z)(Z) 4030 1.04 0.047734 4.00 1.00

Galaxolide (Cis) 4750 0.65 0.037368 0.74 5.94 0.74

Galaxolide (Trans) 4765 0.65 0.037646 0.74 6.00 0.74

Geranial 2665 0.8 0.041155 1.35 1.00

Geraniol 2505 1.395 0.060047 5.01 1.00

Geranyl Acetate 3015 0.585 0.034552 1.15 13.92 14.02 1.00

Hexadecanolide 4955 0.65 0.037108 1.00

Hexyl Cinnamic Aldehyde (E) 4455 0.915 0.04388 2.21 1.00

Hydroxycitronellal 2765 1.47 0.062564 1.00

Hydroxyisohexyl 3-cyclohexene carboxaldehyde

(Cyclohexal / Lyral major) 4265 1.47 0.062262 1.23 1.50 2.24 3.34 1.00

Hydroxyisohexyl 3-cyclohexene carboxaldehyde

(Cyclohexal / Lyral minor) 4240 1.455 0.059895 1.23 2.98 3.16 1.00

Iso E Super Alpha 4190 0.675 0.036123 3.85 6.08 1.00

Iso E Super Beta 4075 0.62 0.037266 1.23 1.25 7.59 1.00

Iso E Super Gamma 4100 0.645 0.037522 1.25 4.96 5.56 7.45 1.00

Iso E Super minor 4050 0.615 0.038151 1.23 4.00 7.70 1.00

Isoeugenol (E) 3520 2.355 0.089013 6.92 1.00

Isoeugenol (Z) 3350 2.155 0.072906 7.59 11.16 1.00

Isoeugenyl Acetate 4165 1.4 0.059352 2.45 2.71 3.51 6.08 1.00

Lilial 3720 0.785 0.042075 1.00

Limonene 1400 0.3 0.038526 1.00

Linalool 1775 0.965 0.047271 1.00

Linalyl Acetate 2405 0.52 0.033467 2.75 3.36 10.91 1.00

Majantol 3290 1.535 0.065928 1.00

Menthol 2140 0.965 0.046888 1.00

Methoxycoumarin-7 4805 2.72 0.10329 1.00

Methyl Eugenol 3335 0.995 0.047454 7.59 1.00

Methyl Heptine Carbonate 2435 0.735 0.039 1.60 2.75 4.16 8.96 1.00

Methyl Octine Carbonate 2815 0.715 0.038717 2.15 2.35 1.00

Methyl Salicylate 2455 1.215 0.054091 4.16 5.37 1.00

Neral 2530 0.77 0.04091 5.01 1.00 n-pentyl isopentyl phthalate 5555 1.065 0.050681 1.00

Phenyl Acetaldehyde 1895 1.335 0.061039 2.41 1.00

Pinene Alpha 970 0.18 0.029529 1.00

Pinene Beta 1195 0.23 0.0377 1.00

Propylidene Phthalide 3- (E) 4080 1.635 0.067658 7.45 7.59 7.70 1.00

Propylidene Phthalide 3- (Z) 4290 1.775 0.065563 0.79 2.24 3.58 0.79

Salicylaldehyde 1865 1.65 0.068457 2.41 1.00

Santalol Alpha 4125 1.195 0.052257 0.71 1.00 1.03 2.38 4.96 0.71

Santalol Beta 4305 1.235 0.055219 3.21 3.58 1.00

Sclareol 5815 1.975 0.080211 1.00

Terpinene Alpha 1350 0.285 0.038326 1.00

Terpineol Alpha 2290 1.03 0.048384 1.24 1.00

Terpineol Beta cis 2065 1.01 0.045621 1.00

Terpineol Beta trans 2180 1.1 0.051334 1.09 4.24 1.00

Terpineol Delta 2200 1.04 0.047463 1.09 3.77 1.00

Terpineol Gamma 2315 1.01 0.047373 1.24 1.00

Terpinolene 1695 0.35 0.033478 1.00

Vanillin 3520 4.545 0.15927 6.92 1.00

Table 8: Example of clustering for Rtx5 x Wax stationary phase combination

Table 9: List of clustered targets

Clustered Defined analytical Rtx-5Sil x Rtx-5Sil x Wax x Rtx-17Sil x VF35 x targets Wax Rtx-17Sil Rtx-5Sil Wax Wax

Amyl Cinnamic Alcohol (E) X X

Anisyl Alcohol X

Carvone X X

Cinnamic Alcohol (E) X

Damascenone Beta X X X

Damascone Alpha (E) X X X X X

Damascone Alpha (Z) X

Damascone Beta (Z) X

Damascone Delta cis/trans X X X X

Damascone Delta trans/trans X X

Diethyl Phthalate X X Estragol X X X

Farnesol (E)(E) X

Farnesol (E)(Z) X X X X

Farnesol (Z)(E) X X X X

Galaxolide (Cis) X X X X X

Galaxolide (Trans) X X X X X

Geranial X X

Geranyl Acetate X

Iso E Super Beta X

Iso E Super minor X

Isoeugenyl Acetate X

Methyl Heptine Carbonate X X

Phenyl Acetaldehyde X

Propylidene Phthalide 3- (E) X

Propylidene Phthalide 3- (Z) X X

Salicylaldehyde X

Terpineol Alpha X X X X

Terpineol Beta trans X X

Terpineol Delta X X X

Terpineol Gamma X X X X

Table 10: Results and parameters of Equations 1, 2, 3, 4 and 5.

Rtx-5Sil Rxi-5Sil x Wax x Rtx- Rtx-17Sil x VF35 x

Parameters in Equation 5, 6 and 7

x Wax Rtx-17Sil 5Sil Wax Wax

First eluting target on first

dimension 1043 1090 605 825 970

Last eluting target on first

dimension ( ) 6251 6300 6905 7095 7010

Modulation period (Pmod) 7 5 5 5 5 Observed first dimension peaks

capacity ( 1,obs nc) 186 261 315 314 302

First eluting target on second

dimension ( 2 t first ) 0.16 0.80 0.49 0.29 0.18

Last eluting target on second

dimension ( 2 t| ast ) 6.62 4.14 4.42 4.60 4.55 a in Equation 7 0.009545 0.004256 0.005142 0.00798 0.00844 b in Equation 7 0.006944 0.018916 0.004442 0.006423 0.006174

Observed second dimension

peaks capacity ( 2,obs nc) 26.2 16.2 24.5 22.7 23.5

Observed 2D dimension peaks

capacity ( obs nc 2D ) 3097 2691 4913 4521 4527

Example 7: Clustering of ingredients Pictorial representations of separation patterns of close defined analytical targets obtained with 2D GC set-ups in accordance with Examples 2 through 6 were prepared and are shown in Figures 2 through 5.