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Determination of nicotine and cotinine in human serum and urine: An interlaboratory study
45
Toxicology Letters, 35 (1987) 45-52 Elsevier
TXL. 01711
DETERMINATION OF NICOTINE AND COTININE AND URINE: AN INTERLABORATORY STUDY*
(Smokers; non-smokers; variation)
radioimmunoassay;
IN HUMAN SERUM
gas chromatography;
interassay
ANTON BIBER”, GERHARD SCHERERb, ILLE HOEPFNERb, FRANZ ADLKOFERb**, DIETER HELLER’, JAMES E. HADDOWd and GEORGE J. KNIGHTd
WOLF-
“Forschungslaboratoriutn Prof. Schievelbein, Munich; bForschungsgesellschaft Rauchen und Gesundheit mbH; Frauenthal2, D 2000 Hamburg 13; ‘Institut fiir Statistik und Mathematische Wirtschaftstheorie der Universitiit Karlsruhe, Karlsruhe (F.R. G.), and dFoundation for Blood Research, Scarborough, ME (U.S.A.) (Received I5 September 1986) (Accepted 25 September 1986)
SUMMARY An interlaboratory study aimed at determining nicotine and cotinine in human serum and urine was carried out. 11 laboratories from 6 countries, all experienced in performing nicotine and cotinine determinations in biological fluids by radioimmunoassay (RIA) and/or gas chromatography (CC) were involved. Each of them received 18 serum and 18 urine samples. The specimens were obtained from 8 smokers and 10 non-smokers; 2 samples from non-smokers were spiked with defined amounts of nicotine and cotinine. All the laboratories distinguished perfectly between the smokers and the non-smokers and according to cotinine levels in serum the laboratories ranked the samples with good agreement. There were systematic differences in the absolute values between the laboratories. The ratios of urinary cotinine concentrations between active and passive smokers differed widely from laboratory to laboratory. The reasons for this are not yet known and necessitate further investigation.
*Presented at the International Experimental Toxicology Symposium on Passive Smoking, October 23-25, 1986, Essen (F.R.G.). **TO whom correspondence and reprint requests should be addressed. Abbreviations: c.v., coefficients of variation; chromatography; RIA, radioimmunoassay.
ETS,
environmental
tobacco
037%4274/87/$ 03.50 0 Elsevier Science Publishers B.V. (Biomedical Division)
smoke;
CC,
gas
46
INTRODUCTION
Nicotine and cotinine in body fluids are often used in order to quantify tobacco smoke uptake. For their determination, GC and RIA methods are normally applied. A controversial discussion in the literature gives rise to some doubt whether data published by different laboratories are comparable with one another [l, 21. The analytical difficulties appear to be most evident in the case of ETS exposure, as very low exposure levels coming close to the detection limit have to be measured. In order to gain further insight into this matter, we initiated an international interlaboratory study. 11 laboratories were involved being experienced in performing nicotine and cotinine determinations in biological fluids by RIA and/or GC.
TABLE
1
NICOTINE
IN SERUM
(ng/ml)
GASCHROMATOGRAPHY
AS MEASURED
X, S and C.V. are calculated -.__
without
the outlying
Laboratories Smoke
Subjects Non-smoker
BY 5 DIFFERENT
A-GC
measurements. -_
D-GC
F-CC
uptake
H-CC
K-CC
6.Sa
co.5
0.4
1.0
0
4.3a
< 0.5
0.2
1.2
3 4
1
?.4a
0.8
0.3
1.5
2
5.?
0.5
0.3
1.3
2 3
5.3 10.1*
0.9 0.6
0.6 0.5
1.8 2.1
3
3 Cig./day 15
Smoker
s
C.V.
-
0
8
x
ETS exp.b
1
6 1
USING
- Methods -.____
2
5
LABORATORIES
(CC)
nd 1
-
-
9.6a
<0.5
0.2
1.8
0.8
0.3
2.1
19
15.0
17.5
18.6
20.4
18.1
2.0
0.11
10
15
7
10.4
9.0
8.8
13.2
9.7
2.3
0.24
11
20
3
ls.oa
1.9
2.3
2.2
2.3
0.5
0.20
12
20
8
14.2
4.8
6.3
8.0
8.3
3.6
0.43
13 14
30 40
11 22
16.7
16.3
4.7
0.29
4.5 4.7
60
32
24.1
32.4
40.0
37.1 40.7
15.1 29.3
0.30
27
15.0 27.7
15.8
40
14.3 12.9 25.0
15.8
15 16
23.1 9.9 29.8
33.8
6.8
0.20
17c
39
26.8
35.4
44.9
44.1
38.0
7.4
0.19
18’
15
17.3
17.5
21.8 _
21.9
18.7
3.0
0.16
9
nd, not detectable. “Outlier. bETS exposure: 0, none; ‘Serum
spiked
1, low; 2, medium;
with 41 and 20 ngiml
nicotine,
3, high. respectively.
0.16
41
MATERIALS
AND
METHODS
Urine obtained from 8 non-smokers and 8 smokers was collected for 24 h, and blood was drawn between 4 and 6 pm at the Forschungslaboratorium Prof. Schievelbein. 6 of the non-smokers reported exposure to ETS. The urine and serum specimens were aliquoted and stored at -20°C. In addition, 2 serum and 2 urine samples derived from non-exposed non-smokers were spiked with nicotine and cotinine. In total, there were 18 urine and 18 serum samples. The frozen specimens (4 ml serum and 10 ml urine) were dispatched on dry ice. The participating laboratories were sent the samples under a code number. Each laboratory could choose its own analytical method. They were asked to return one single value for nicotine and cotinine from each sample.
TABLE
II
NICOTINE
IN URINE
(ng/mI)
AS MEASURED
GASCHROMATOGRAPHY
(CC)
X, S and C.V. are calculated
without
the outlying
Laboratories Smoke
Subjects
BY 5 DIFFERENT
LABORATORIES
USING
measurements.
- Methods
A-CC
D-W
I-GC
F-GC
K-GC
X
S
C.V.
uptake Non-smoker
ETS exp.b
1
0
4
nd
8.3
<5
7.1
2
0
7
5
4.0
16.0
3
6.2
3
1
nd
4.5
26 <5
4
2
<3
nd
4.9
450a
5
2
<3
nd
2.4
<5
6
3
<3
nd
4.9
38
15.9
I
3
9
nd
5.6
8
3
32
nd
19.9
28 540a
34.0
2.3 8.4 8.2
Cig./day
Smoker 9
15
149
124
150
190
153
27
0.18
10
15
1191
907
1190
345
1189
11
20
255
186
154
118
204
964 183
367 51
0.38 0.28 0.04 0.16
51Sa
12
20
861a
615
609
650
650
631
22
13
30
519
459
450
338
500
453
70
14
40
1333
1155
1092
1320
627
1105
286
0.26
15
40
3218
2967
3331
3198
3125
3168
134
0.04
16
60
3279
3417
3486
2813
3391
3277
270
0.08
2687 1404
2483 1112
2599
1365= 1025
2601 1269
2592
83
0.03
1233
161
0.13
11’ 18’ aOutlier.
nd, not detectable.
bETS exposure: ‘Urine
1356
spiked
0, none;
1, low; 2, medium;
with 2500 and 1200 ng/ml
3, high.
nicotine,
respectively.
48 RESULTS AND DISCUSSION
Only 5 laboratories were able to measure nicotine in serum and in urine, all of them using GC. Cotinine in serum and urine were each determined by 10 laboratories. The results are summarized in Tables I to IV. The recovery rates calculated from the spiked serum and urine samples ranged from 55 to 117% for NICOTINE
IN SERUM (NC/ML.)
‘ik
'ik
NICOTINE
IN URINE (NC/ML)
7000
2000
f-
k-lx D-SC F-6C H-BC
4.5 4.8 . 0 1.4
K-SC
. 0
3000
F-GE I-GC x-Gc
-0 403 230
1500
/ ’
cI IO
20 COTININE
‘ik
A-RIA
IN SERUX
‘k
40
30 (NG,‘ML)
^
”
(NG/M,,)
48
600 E-RIA
COTININE IN URINE
X ,k
iooo
42
8-RIA C-RIP.
50 26
E-RIA
349
5000 300
0
0
200
400
600
80
3000
6000
9000
Fig. 1. Linear model (according to Jaech [3]) based on the samples from smokers and on the spiked samples (n = 10). Model, Xik7
Pk, @i, I%), Eik,
u,
Xik = ai + pi . pk + EI~;i = 1, . . . , 11; k = 9, ..* , 18. measurement value for sample k, derived by laboratory i. true but unknown value for sample k. bias for laboratory i. error term with expectation 0 and variance bi2 diagonal line in plots.
III
IN SERUM
Smoke
2
2
3
3
3
4
5
6
7
8
30
40
40
60
13
14
15
16
‘Serum
0, none;
249
478 42.Sa
95.0”
120.6”
105.8”
54.2a
53.3”
41.0a
11.7
12.0=
39.7
nd
0.4
0.2
nd
nd
nd
nd
nd
C-RIA
respectively.
3, high.
cotinine,
1, low; 2, medium;
224
463
697
631
706
670
741
325
234
63
90
211
620
289
229
75
107
260
334
spiked with 420 and 210 rig/ml
bETS exposure:
“Outlier.
nd, not detectable.
1.9 4.9
1
4
6.4
0.9
0.8
2.0
0.6
0.6
B-RIA
6
<1
<1
<1
A-GC
- Methods
measurements.
220
460
481
680
260
370
197
40
84
196
5.1
nd
7.7
3.0
2.3
6.4”
3.0”
8.6
D-CC
BY 10 DIFFERENT
354
357
330
338
223
20
12
60
457
20
11
80
228
4
2
6
2
2
1
17c
15
IO
18’
15
9
Cig./day
1
3
Smoker
0
0
A-RIA
Laboratories
the outlying
AS MEASURED
without
(GC)
(ng/ml)
ETS exp.b
uptake
2
Non-smoker 1
Subjects
x, s and C.V. are calculated
CHROMATOGRAPHY
COTININE
TABLE
208
388
382
449
263
289
199
40
65
119
nd
nd
nd
nd
nd
nd
nd
nd
E-RIA
2
3
4
4
2
185
398
527
587
261
250
157
31
73
179
<1
F-CC
LABORATORIES
165
330
480
168
351
347 198
399 196
183
525 467
529
205
407
542
585
544
24
54
104
92
50
51
278 278
54
202
19
14 42
58 76
s
176
x
(RIA) AND/OR
231
251 498
255
228
14
51
175
<1
<1
L-RIA
555
251
222 510
242
172
42
45 179
67
171
3.5
2.4
5.5
0.5
0.6
1.4
0.8
0.5
K-CC
75
198
2.1
0.4
2.5
0.2
1.4
H-CC
RADIOIMMUNOASSAY
210
155
47
67
16.5
nd
nd
15
nd
28’
nd
nd
62’
G-GC
USING
0.12
0.13
0.19
0.16
0.18
0.18
0.27
0.45
0.19
0.33
C.V.
GAS
IV
IN URINE
3
3
3
8
‘Urine
0, none;
3.9
14.5
75.0
16.0
4970
respectively.
795a
1645”
3573
7464
3193
10240
2253
486 671a
3490 4120
700
1145 1393
232
302
205
512
173 66
1150
268
nd
nd
nd
nd
nd
nd
43
nd
D-GC
347
2550
2015
2630
425
140
45.9
nd
36.1
2.6 45.0
3.1
nd
4.0
18.2
4.4
4.5
13.0
1635
3, high.
cotinine,
1, low; 2, medium;
spiked with 8700 and 4400 ng/ml
bETS exposure:
nd, not detectable. “Outlier.
8623
4120
3512
2536
8478
5245
4040
4088
60
16
1736
1124
1749
324
1014
1298
38
2
2
17c
40
15
3726
3726a
5196”
626
1002
2153
150a
11
17a
5
18’
30
20
12
40
20
11
14
15
10
13
15
9
Cig./day
19
31
2
5
6 I
Smoker
38
76
2
4
17a
2
1
13
3
7
0
25
0
B-RIA
C-RIA
measurements.
BY 10 DIFFERENT
- Methods
A-GC
Laboratories
A-RIA
2
ETS exp.b
uptake
Smoke
1
Non-smoker
Subjects
the outlying
AS MEASURED
without
(GC)
(rig/ml)
x, s and C.V. are calculated
CHROMATOGRAPHY
COTININE
TABLE
3834
8774
2960
2355
1823
2919
301
1080
1541
61
nd
44
nd
nd
nd
nd
nd
E-RIA
4159
8236
2833
2091
703
732
1002
129
460
878
15
9
21
2
7
4
10
18
F-GC
LABORATORIES
4270
8710
3280
2430
1570
940
1590
190
720
1370
H-GC
USING
4108
3278
1565
1750
690
1420
178
903
880
61
12
19
3oa
8
26 7
18
I-GC
1.0
8500 4242
7997 4018
3718
2604
2416
1474
2580
260
538
1236
29.1
3.8
12.6
4.0
<1
L-RIA
2920
2270
745
899
1091
201
605
1050
21.4
8.5
30.6
3.6
2.9
4.9
15.7
3.4
K-GC
RADIOIMMUNOASSAY
4138
8442
3566
2429
1754
1063
1648
264
704
1223
x
357
798
742
934
979
554
847
154
219
484
s
(RIA) AND/OR
0.09
0.09
0.21
0.38
0.56
0.52
0.51
0.59
0.40
0.40
C.V.
GAS
nicotine, and from 79-I 19% for cotinine. There were no differences in recovery rates between the urine and serum samples. The data from laboratory C were excluded from this calculation, as they show a recovery rate for cotinine of about 20% only. In the samples obtained from smokers the interlaboratory C.V. ranged from 4 to 59%. They were not influenced by increasing cigarette consumption. With regard to nicotine, the coefficients of variation were similar when the measurements were made in serum or urine, whereas for cotinine the mean coefficient of variation in urine was twice as high as found in serum. This is due to the fact that cotinine determinations in urine by RIA are less precise than in serum. For the spiked samples the coefficients of variation ranged from 3 to 19% being much lower than in the samples from smokers. As yet we have no explanation for this. The coefficients of variation for the samples obtained from non-smokers should not be calculated, since most of the values are below the detection limit and no numerical figures are available. The ratios of urinary cotinine concentrations between active and passive smokers differed widely ranging from 21 in laboratory C to 294 in laboratory L. In order to describe the results of the interlaboratory study in a more condensed form, a linear model [3] based on the samples obtained from smokers and on the spiked samples was used (Fig. 1). A comparison of the model line obtained from each laboratory with the ideal line (diagonal) indicates the degree of deviation of the laboratory’s results. A low u-value means high precision. Cotinine values in serum are comparable whether determined by RIA or GC, whereas in urine the RIA values are higher than the GC values. The data obtained in laboratory C have been disregarded. The results of our interlaboratory study indicate that data on nicotine and cotinine concentrations in serum and urine from smokers published so far are certainly comparable on a relative basis (coefficient of correlation: 0.6-0.9). In general, the laboratories ranked the samples according to cotinine levels in serum with good agreement. The absolute values, however, show large interlaboratory variations. These are particularly high in the samples obtained from subjects exposed to ETS. ACKNOWLEDGEMENTS
The study was carried out in the following laboratories: Dr. N. Benowitz, Clinical Pharmacology Unit, General Hospital Center, San Francisco (U.S.A.); Dr. A. Biber, Forschungslaboratorium Prof. Schievelbein, Munich (F.R.G.); Dr. M. Curvall, Swedish Tobacco Co, Stockholm (Sweden); Dr. C. Feyerabend, Dr, M.A.H. Russell, Institute of Psychiatry, University of London, London (U.K.); Dr. J.E. Haddow, Dr. GE. Knight, Foundation for Blood Research, Scarborough, ME (U.S.A.); Dr. N.J. Haley, American Health Foundation, New York (U.S.A.); Dr. S. Matsukura, Miyazaki Medical College, Kiyotake (Japan); Dr. H. Muranaka, Kyoto Senbai Hospital, Kyoto (Japan); Dr. H. Nau, Institut fur Toxikologie und
52
Embryonalpharmakologie, Freie Universitat Berlin, Berlin (Germany); Dr. K. Engstrom; Dr. M. Sorsa, Institute of Occupational Health, Helsinki (Finland); Dr. N. Wald, Medical College of St. Bartholomew’s Hospital, London (U.K.). The authors are indebted to all the scientists participating in this study. Without their spontaneous cooperation it would not have been possible to carry out this investigation.
REFERENCES 1 S. Matsukura, Y. Hirata, Evidence
Jaech,
0.
K. Norikazu,
of environmental
for passive
2 F. Adlkofer, 719-720. 3 J.L.
T. Tomohiko, Effects
smoking,
Scherer
Statistical
S. Yutaka,
tobacco
N. Engl.
J. Med.,
and U. von Hees,
Analysis
smoke
M. Uchihashi, cotinine
H. Nakajima
excretion
and
in nonsmokers.
311 (1984) 828-832.
Passive
of Measurement
H. Hamada, on urinary smoking
Errors,
(Letter),
Wiley,
N. Engl.
New York,
J. Med.,
1985.
312 (1985)
Toxicology Letters, 35 (1987) 45-52 Elsevier
TXL. 01711
DETERMINATION OF NICOTINE AND COTININE AND URINE: AN INTERLABORATORY STUDY*
(Smokers; non-smokers; variation)
radioimmunoassay;
IN HUMAN SERUM
gas chromatography;
interassay
ANTON BIBER”, GERHARD SCHERERb, ILLE HOEPFNERb, FRANZ ADLKOFERb**, DIETER HELLER’, JAMES E. HADDOWd and GEORGE J. KNIGHTd
WOLF-
“Forschungslaboratoriutn Prof. Schievelbein, Munich; bForschungsgesellschaft Rauchen und Gesundheit mbH; Frauenthal2, D 2000 Hamburg 13; ‘Institut fiir Statistik und Mathematische Wirtschaftstheorie der Universitiit Karlsruhe, Karlsruhe (F.R. G.), and dFoundation for Blood Research, Scarborough, ME (U.S.A.) (Received I5 September 1986) (Accepted 25 September 1986)
SUMMARY An interlaboratory study aimed at determining nicotine and cotinine in human serum and urine was carried out. 11 laboratories from 6 countries, all experienced in performing nicotine and cotinine determinations in biological fluids by radioimmunoassay (RIA) and/or gas chromatography (CC) were involved. Each of them received 18 serum and 18 urine samples. The specimens were obtained from 8 smokers and 10 non-smokers; 2 samples from non-smokers were spiked with defined amounts of nicotine and cotinine. All the laboratories distinguished perfectly between the smokers and the non-smokers and according to cotinine levels in serum the laboratories ranked the samples with good agreement. There were systematic differences in the absolute values between the laboratories. The ratios of urinary cotinine concentrations between active and passive smokers differed widely from laboratory to laboratory. The reasons for this are not yet known and necessitate further investigation.
*Presented at the International Experimental Toxicology Symposium on Passive Smoking, October 23-25, 1986, Essen (F.R.G.). **TO whom correspondence and reprint requests should be addressed. Abbreviations: c.v., coefficients of variation; chromatography; RIA, radioimmunoassay.
ETS,
environmental
tobacco
037%4274/87/$ 03.50 0 Elsevier Science Publishers B.V. (Biomedical Division)
smoke;
CC,
gas
46
INTRODUCTION
Nicotine and cotinine in body fluids are often used in order to quantify tobacco smoke uptake. For their determination, GC and RIA methods are normally applied. A controversial discussion in the literature gives rise to some doubt whether data published by different laboratories are comparable with one another [l, 21. The analytical difficulties appear to be most evident in the case of ETS exposure, as very low exposure levels coming close to the detection limit have to be measured. In order to gain further insight into this matter, we initiated an international interlaboratory study. 11 laboratories were involved being experienced in performing nicotine and cotinine determinations in biological fluids by RIA and/or GC.
TABLE
1
NICOTINE
IN SERUM
(ng/ml)
GASCHROMATOGRAPHY
AS MEASURED
X, S and C.V. are calculated -.__
without
the outlying
Laboratories Smoke
Subjects Non-smoker
BY 5 DIFFERENT
A-GC
measurements. -_
D-GC
F-CC
uptake
H-CC
K-CC
6.Sa
co.5
0.4
1.0
0
4.3a
< 0.5
0.2
1.2
3 4
1
?.4a
0.8
0.3
1.5
2
5.?
0.5
0.3
1.3
2 3
5.3 10.1*
0.9 0.6
0.6 0.5
1.8 2.1
3
3 Cig./day 15
Smoker
s
C.V.
-
0
8
x
ETS exp.b
1
6 1
USING
- Methods -.____
2
5
LABORATORIES
(CC)
nd 1
-
-
9.6a
<0.5
0.2
1.8
0.8
0.3
2.1
19
15.0
17.5
18.6
20.4
18.1
2.0
0.11
10
15
7
10.4
9.0
8.8
13.2
9.7
2.3
0.24
11
20
3
ls.oa
1.9
2.3
2.2
2.3
0.5
0.20
12
20
8
14.2
4.8
6.3
8.0
8.3
3.6
0.43
13 14
30 40
11 22
16.7
16.3
4.7
0.29
4.5 4.7
60
32
24.1
32.4
40.0
37.1 40.7
15.1 29.3
0.30
27
15.0 27.7
15.8
40
14.3 12.9 25.0
15.8
15 16
23.1 9.9 29.8
33.8
6.8
0.20
17c
39
26.8
35.4
44.9
44.1
38.0
7.4
0.19
18’
15
17.3
17.5
21.8 _
21.9
18.7
3.0
0.16
9
nd, not detectable. “Outlier. bETS exposure: 0, none; ‘Serum
spiked
1, low; 2, medium;
with 41 and 20 ngiml
nicotine,
3, high. respectively.
0.16
41
MATERIALS
AND
METHODS
Urine obtained from 8 non-smokers and 8 smokers was collected for 24 h, and blood was drawn between 4 and 6 pm at the Forschungslaboratorium Prof. Schievelbein. 6 of the non-smokers reported exposure to ETS. The urine and serum specimens were aliquoted and stored at -20°C. In addition, 2 serum and 2 urine samples derived from non-exposed non-smokers were spiked with nicotine and cotinine. In total, there were 18 urine and 18 serum samples. The frozen specimens (4 ml serum and 10 ml urine) were dispatched on dry ice. The participating laboratories were sent the samples under a code number. Each laboratory could choose its own analytical method. They were asked to return one single value for nicotine and cotinine from each sample.
TABLE
II
NICOTINE
IN URINE
(ng/mI)
AS MEASURED
GASCHROMATOGRAPHY
(CC)
X, S and C.V. are calculated
without
the outlying
Laboratories Smoke
Subjects
BY 5 DIFFERENT
LABORATORIES
USING
measurements.
- Methods
A-CC
D-W
I-GC
F-GC
K-GC
X
S
C.V.
uptake Non-smoker
ETS exp.b
1
0
4
nd
8.3
<5
7.1
2
0
7
5
4.0
16.0
3
6.2
3
1
nd
4.5
26 <5
4
2
<3
nd
4.9
450a
5
2
<3
nd
2.4
<5
6
3
<3
nd
4.9
38
15.9
I
3
9
nd
5.6
8
3
32
nd
19.9
28 540a
34.0
2.3 8.4 8.2
Cig./day
Smoker 9
15
149
124
150
190
153
27
0.18
10
15
1191
907
1190
345
1189
11
20
255
186
154
118
204
964 183
367 51
0.38 0.28 0.04 0.16
51Sa
12
20
861a
615
609
650
650
631
22
13
30
519
459
450
338
500
453
70
14
40
1333
1155
1092
1320
627
1105
286
0.26
15
40
3218
2967
3331
3198
3125
3168
134
0.04
16
60
3279
3417
3486
2813
3391
3277
270
0.08
2687 1404
2483 1112
2599
1365= 1025
2601 1269
2592
83
0.03
1233
161
0.13
11’ 18’ aOutlier.
nd, not detectable.
bETS exposure: ‘Urine
1356
spiked
0, none;
1, low; 2, medium;
with 2500 and 1200 ng/ml
3, high.
nicotine,
respectively.
48 RESULTS AND DISCUSSION
Only 5 laboratories were able to measure nicotine in serum and in urine, all of them using GC. Cotinine in serum and urine were each determined by 10 laboratories. The results are summarized in Tables I to IV. The recovery rates calculated from the spiked serum and urine samples ranged from 55 to 117% for NICOTINE
IN SERUM (NC/ML.)
‘ik
'ik
NICOTINE
IN URINE (NC/ML)
7000
2000
f-
k-lx D-SC F-6C H-BC
4.5 4.8 . 0 1.4
K-SC
. 0
3000
F-GE I-GC x-Gc
-0 403 230
1500
/ ’
cI IO
20 COTININE
‘ik
A-RIA
IN SERUX
‘k
40
30 (NG,‘ML)
^
”
(NG/M,,)
48
600 E-RIA
COTININE IN URINE
X ,k
iooo
42
8-RIA C-RIP.
50 26
E-RIA
349
5000 300
0
0
200
400
600
80
3000
6000
9000
Fig. 1. Linear model (according to Jaech [3]) based on the samples from smokers and on the spiked samples (n = 10). Model, Xik7
Pk, @i, I%), Eik,
u,
Xik = ai + pi . pk + EI~;i = 1, . . . , 11; k = 9, ..* , 18. measurement value for sample k, derived by laboratory i. true but unknown value for sample k. bias for laboratory i. error term with expectation 0 and variance bi2 diagonal line in plots.
III
IN SERUM
Smoke
2
2
3
3
3
4
5
6
7
8
30
40
40
60
13
14
15
16
‘Serum
0, none;
249
478 42.Sa
95.0”
120.6”
105.8”
54.2a
53.3”
41.0a
11.7
12.0=
39.7
nd
0.4
0.2
nd
nd
nd
nd
nd
C-RIA
respectively.
3, high.
cotinine,
1, low; 2, medium;
224
463
697
631
706
670
741
325
234
63
90
211
620
289
229
75
107
260
334
spiked with 420 and 210 rig/ml
bETS exposure:
“Outlier.
nd, not detectable.
1.9 4.9
1
4
6.4
0.9
0.8
2.0
0.6
0.6
B-RIA
6
<1
<1
<1
A-GC
- Methods
measurements.
220
460
481
680
260
370
197
40
84
196
5.1
nd
7.7
3.0
2.3
6.4”
3.0”
8.6
D-CC
BY 10 DIFFERENT
354
357
330
338
223
20
12
60
457
20
11
80
228
4
2
6
2
2
1
17c
15
IO
18’
15
9
Cig./day
1
3
Smoker
0
0
A-RIA
Laboratories
the outlying
AS MEASURED
without
(GC)
(ng/ml)
ETS exp.b
uptake
2
Non-smoker 1
Subjects
x, s and C.V. are calculated
CHROMATOGRAPHY
COTININE
TABLE
208
388
382
449
263
289
199
40
65
119
nd
nd
nd
nd
nd
nd
nd
nd
E-RIA
2
3
4
4
2
185
398
527
587
261
250
157
31
73
179
<1
F-CC
LABORATORIES
165
330
480
168
351
347 198
399 196
183
525 467
529
205
407
542
585
544
24
54
104
92
50
51
278 278
54
202
19
14 42
58 76
s
176
x
(RIA) AND/OR
231
251 498
255
228
14
51
175
<1
<1
L-RIA
555
251
222 510
242
172
42
45 179
67
171
3.5
2.4
5.5
0.5
0.6
1.4
0.8
0.5
K-CC
75
198
2.1
0.4
2.5
0.2
1.4
H-CC
RADIOIMMUNOASSAY
210
155
47
67
16.5
nd
nd
15
nd
28’
nd
nd
62’
G-GC
USING
0.12
0.13
0.19
0.16
0.18
0.18
0.27
0.45
0.19
0.33
C.V.
GAS
IV
IN URINE
3
3
3
8
‘Urine
0, none;
3.9
14.5
75.0
16.0
4970
respectively.
795a
1645”
3573
7464
3193
10240
2253
486 671a
3490 4120
700
1145 1393
232
302
205
512
173 66
1150
268
nd
nd
nd
nd
nd
nd
43
nd
D-GC
347
2550
2015
2630
425
140
45.9
nd
36.1
2.6 45.0
3.1
nd
4.0
18.2
4.4
4.5
13.0
1635
3, high.
cotinine,
1, low; 2, medium;
spiked with 8700 and 4400 ng/ml
bETS exposure:
nd, not detectable. “Outlier.
8623
4120
3512
2536
8478
5245
4040
4088
60
16
1736
1124
1749
324
1014
1298
38
2
2
17c
40
15
3726
3726a
5196”
626
1002
2153
150a
11
17a
5
18’
30
20
12
40
20
11
14
15
10
13
15
9
Cig./day
19
31
2
5
6 I
Smoker
38
76
2
4
17a
2
1
13
3
7
0
25
0
B-RIA
C-RIA
measurements.
BY 10 DIFFERENT
- Methods
A-GC
Laboratories
A-RIA
2
ETS exp.b
uptake
Smoke
1
Non-smoker
Subjects
the outlying
AS MEASURED
without
(GC)
(rig/ml)
x, s and C.V. are calculated
CHROMATOGRAPHY
COTININE
TABLE
3834
8774
2960
2355
1823
2919
301
1080
1541
61
nd
44
nd
nd
nd
nd
nd
E-RIA
4159
8236
2833
2091
703
732
1002
129
460
878
15
9
21
2
7
4
10
18
F-GC
LABORATORIES
4270
8710
3280
2430
1570
940
1590
190
720
1370
H-GC
USING
4108
3278
1565
1750
690
1420
178
903
880
61
12
19
3oa
8
26 7
18
I-GC
1.0
8500 4242
7997 4018
3718
2604
2416
1474
2580
260
538
1236
29.1
3.8
12.6
4.0
<1
L-RIA
2920
2270
745
899
1091
201
605
1050
21.4
8.5
30.6
3.6
2.9
4.9
15.7
3.4
K-GC
RADIOIMMUNOASSAY
4138
8442
3566
2429
1754
1063
1648
264
704
1223
x
357
798
742
934
979
554
847
154
219
484
s
(RIA) AND/OR
0.09
0.09
0.21
0.38
0.56
0.52
0.51
0.59
0.40
0.40
C.V.
GAS
nicotine, and from 79-I 19% for cotinine. There were no differences in recovery rates between the urine and serum samples. The data from laboratory C were excluded from this calculation, as they show a recovery rate for cotinine of about 20% only. In the samples obtained from smokers the interlaboratory C.V. ranged from 4 to 59%. They were not influenced by increasing cigarette consumption. With regard to nicotine, the coefficients of variation were similar when the measurements were made in serum or urine, whereas for cotinine the mean coefficient of variation in urine was twice as high as found in serum. This is due to the fact that cotinine determinations in urine by RIA are less precise than in serum. For the spiked samples the coefficients of variation ranged from 3 to 19% being much lower than in the samples from smokers. As yet we have no explanation for this. The coefficients of variation for the samples obtained from non-smokers should not be calculated, since most of the values are below the detection limit and no numerical figures are available. The ratios of urinary cotinine concentrations between active and passive smokers differed widely ranging from 21 in laboratory C to 294 in laboratory L. In order to describe the results of the interlaboratory study in a more condensed form, a linear model [3] based on the samples obtained from smokers and on the spiked samples was used (Fig. 1). A comparison of the model line obtained from each laboratory with the ideal line (diagonal) indicates the degree of deviation of the laboratory’s results. A low u-value means high precision. Cotinine values in serum are comparable whether determined by RIA or GC, whereas in urine the RIA values are higher than the GC values. The data obtained in laboratory C have been disregarded. The results of our interlaboratory study indicate that data on nicotine and cotinine concentrations in serum and urine from smokers published so far are certainly comparable on a relative basis (coefficient of correlation: 0.6-0.9). In general, the laboratories ranked the samples according to cotinine levels in serum with good agreement. The absolute values, however, show large interlaboratory variations. These are particularly high in the samples obtained from subjects exposed to ETS. ACKNOWLEDGEMENTS
The study was carried out in the following laboratories: Dr. N. Benowitz, Clinical Pharmacology Unit, General Hospital Center, San Francisco (U.S.A.); Dr. A. Biber, Forschungslaboratorium Prof. Schievelbein, Munich (F.R.G.); Dr. M. Curvall, Swedish Tobacco Co, Stockholm (Sweden); Dr. C. Feyerabend, Dr, M.A.H. Russell, Institute of Psychiatry, University of London, London (U.K.); Dr. J.E. Haddow, Dr. GE. Knight, Foundation for Blood Research, Scarborough, ME (U.S.A.); Dr. N.J. Haley, American Health Foundation, New York (U.S.A.); Dr. S. Matsukura, Miyazaki Medical College, Kiyotake (Japan); Dr. H. Muranaka, Kyoto Senbai Hospital, Kyoto (Japan); Dr. H. Nau, Institut fur Toxikologie und
52
Embryonalpharmakologie, Freie Universitat Berlin, Berlin (Germany); Dr. K. Engstrom; Dr. M. Sorsa, Institute of Occupational Health, Helsinki (Finland); Dr. N. Wald, Medical College of St. Bartholomew’s Hospital, London (U.K.). The authors are indebted to all the scientists participating in this study. Without their spontaneous cooperation it would not have been possible to carry out this investigation.
REFERENCES 1 S. Matsukura, Y. Hirata, Evidence
Jaech,
0.
K. Norikazu,
of environmental
for passive
2 F. Adlkofer, 719-720. 3 J.L.
T. Tomohiko, Effects
smoking,
Scherer
Statistical
S. Yutaka,
tobacco
N. Engl.
J. Med.,
and U. von Hees,
Analysis
smoke
M. Uchihashi, cotinine
H. Nakajima
excretion
and
in nonsmokers.
311 (1984) 828-832.
Passive
of Measurement
H. Hamada, on urinary smoking
Errors,
(Letter),
Wiley,
N. Engl.
New York,
J. Med.,
1985.
312 (1985)