CA2065924C - Method for detecting maternally transferred drug metabolites in newborn infants - Google Patents
Method for detecting maternally transferred drug metabolites in newborn infantsInfo
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- CA2065924C CA2065924C CA 2065924 CA2065924A CA2065924C CA 2065924 C CA2065924 C CA 2065924C CA 2065924 CA2065924 CA 2065924 CA 2065924 A CA2065924 A CA 2065924A CA 2065924 C CA2065924 C CA 2065924C
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Abstract
An improved method for detecting the presence of drug metabolites in the meconium of newborn infants is described. The method involves a single step extraction of the drug metabolites from meconium using a buffered aqueous solution containing methanol in an amount between about 10 and 30 % by volume and buffered to a pH between 6 and 7 and then assaying the extract individually for the presence of the drug metabolites. The method is particularly useful for detection of cocaine, morphine, cannabinoid and amphetamine metabolites; however, any drug metabolite in the infant meconium can be tested if it is extracted by the solution from the meconium. Various assay methods are used for the drug metabolites in the solutions derived from the meconium, including immunoassays, fluorescent assays and mass spectroscopy. The method provides a means for early detection of drug presence in newborn infants which contribute to infant illness.
Description
20659~4 WSU 4.1-51 IMPROVED METHOD FOR DETECTING MATERNALLY
TRANSFERRED DRUG METABOLITES IN NEWBORN INFA~TS
Cross-Reference to Related Application This application is related to Canadian aDDli~tion Serial No. 2,001,229 filed October 23, 1989.
BACKGROUND OF THE INVENTION
S (1) Summary of the Invention The present invention relates to an improved method for detecting drug metabolites which are transferred from a mother to a newborn in~ant during pregnancy. In particular, the method involves the isolation of meconium from a newborn infant, separation of the drug metabolites from the meconium in a single solution and assaying for the metabolites in the solution.
TRANSFERRED DRUG METABOLITES IN NEWBORN INFA~TS
Cross-Reference to Related Application This application is related to Canadian aDDli~tion Serial No. 2,001,229 filed October 23, 1989.
BACKGROUND OF THE INVENTION
S (1) Summary of the Invention The present invention relates to an improved method for detecting drug metabolites which are transferred from a mother to a newborn in~ant during pregnancy. In particular, the method involves the isolation of meconium from a newborn infant, separation of the drug metabolites from the meconium in a single solution and assaying for the metabolites in the solution.
(2) Prior Art The use of illicit drugs in the United States is widespread. According to a national survey in 1985, an estimated 23 million people were users of illicit drugs (1985 National Health Household Survey on Drug Abuse.
Rockville, MD., 1987). Although exact figures are not known, a sizable portion of drug users are women of childbearing age or are pregnant women. Infants born to these drug dependent women have multiple problems. In the neonatal period, their mortality rate is increased as well as morbidity, which includes asphyxia, prematurity, low birth weight, hyaline membrane disease, infections, aspiration pneumonia, congenital malformations, abnormal heart rate and breathing patterns and drug withdrawal (Ostrea, E. M., Chavez, C. J., J. Pediatr. 94:292-295, (1979); Zelson, C., Rubio E., and Wasserman, E., Pediatrics 48:178 (1971)). Long term sequelae are not uncommon and include delays in physical growth and mental development, -2- ~ 2 4 ~
sudden infant death syndrome, hyperactivity, ocular and neurologic abnormalities and lately, a risk to acquired immunodeficiency disease (Wilson, G. S., McCreary, M., Kean, J., and Baxter, J., Pediatrics 63:135-144 (1979);
Chavez, C. J., et al., J. Pediatrics 95:407-409 (1979);
Chasnoff, I. J., et al., Pediatrics 70:210-213 (1982);
Chavez, C. J., et al., Pediatr. Res. 12:367A, (1979); and oleske, J., et al., J. Am. Med. Assoc., 249:2345-2349 (1983)). At present, cocaine abuse among pregnant women has also become widespread and infant morbidity, notably cerebrovascular problems have been reported (Chasnoff, I.
J., et al., J. Pediatr. 108:456-459 (1986)). Because of these immediate and long term problems, infants of drug dependent mothers (IDDM) constitute a high risk group and lS have to be identified as soon as possible after birth if intervention is to be successful.
Unfortunately, the identification of the drug exposed neonate is not easy. Many of the drugs to which the fetus is exposed, in utero, do not produce immediate or recognizable effects in the neonates (Kandall, S. R., Am.
J. Dis. Child, 127:58-61 (1974)). Maternal admission of drug usage is often inaccurate because of fear of the consequences stemming from such admission. Eve~n with maternal cooperation, such information regarding the type and extent of drug usage is often inaccurate (Ostrea, E.
M., et al., J. Pediatr. 88:642-645 (1976)). One alternative is to test the infant's urine for drugs, but this procedure has its limitations since successful detection of drug metabolites in the infant's urine is dependent on time of the last drug intake by the mother or when, after birth, the infant's urine was collected. A
high rate of false negative results in neonatal urine tests can arise from the mother's abstention from the use of the drug a few days before she delivers or to the inability to obtain a sample of the infant's urine soon after birth (Halstead, A. C., et al., Clin. Biochem. 21:59-61 (1988)).
Our experience verifies this diagnostic problem. Urine ,, from 337 infants of known drug dependent mothers was tested by thin-layer chromatography. It was found that only 13%
were positive. Similarly, only 37% of the urine samples taken from drug dependent infants were positive for drugs when tested by TDX fluorescent polarization immunoassay (Ostrea, E. M., Brady, M. J., Parks, P. M., Asensio, D. C., Nalaz, A., J. Ped. 115:474-474 (1989) ). Even with more sensi~ive methods such as radioimmunoassay, 8 urine samples tested negative for drugs despite a positive test in the stools (Ostrea, E. M., ~rady, M. J., Parks, P. M., Asensio, D. C., Naluz, A., J. Ped. 115:474-474 (~1989)). Clearly, there is a need for a better way to detect prenatal drug exposure in this high risk group of infants.
A new method has been developed for identifying fetal drug exposure by detecting drug metabolites in meconium, the first green stools of the newborn infant which is passed within a few days after birth (Ostrea, E.
M., Parks, P., Brady, M., Clin. Chem. 34:2372-2373 (1989);
Ostrea, E. M., Brady, M. J., Parks, P. M., Asensio, D. C., Naluz, A., J. Ped. 115:474-474 tl989) ) . The concept behind this method was based on initial research in pregnant, morphine addicted monkeys (Ostrea, E. M., Lynn, S. N., Wayne, R. H., Stryker, J. C., Dev. Pharmacol. Ther. 9 80;
1:163-170 (1980) ) and subsequently in rats (Ostrea, E. M., Brady, M. J., Parks, P. M., Asensio, D. C., Naluz, A., J.
Ped. 115:474-477 (1989) ) which showed that a high concentration of drug metabolites were present in the gastrointestinal tract of their fetuses. we interpreted this observation to be a consequence of the following mechanism: morphine in the fetus is metabolized by the liver to water soluble glucuronide conjuga~es which are then excreted into the bile or urine (Jaffe, J., Drug addiction and drug abuse. In: Goodman, L., Gillman, A., eds. The Pharmacologic Basis of Therapeutics. London:
Collier-Macmillan, 535-584 (1989)). In either case, morphine glucuronide accumulates in the fetal intestines either from bile secretion or from fetal urine which is 206592~
swallowed via the amniotic fluid. Thus, meconium represents an excretion product which is cumulative of the entire gestation. Overall therefore, meconium acts as a reservoir of drug metabolites in the fetus; seemingly a stockpile of pharmacologic waste products throughout gestation.
Clinical studies have been conducted which have validated meconium analysis as a reliable drug screen in the newborn infant:
1. Meconium obtained from 20 infants of drug-dependent mothers and five control infants were analyzed by radioimmunoassay for the metabolites of heroin, cocaine and cannabinoids (Ostrea, E. M., Brady, M. J., Parks, P. M., Asensio, D. C., Naluz, A., J. Ped.
115-474-477 (1989)). Control stools showed no drug.
Meconium from the infants of drug-dependent mothers showed the presence of at least one drug metabolite: 80% of the infants of drug-dependent mothers showed cocaine (range 0.14 to 19.91 ~g/g stool), 55% showed morphine (range 0.41 to 14.97 ~g/g stool), and 60% showed cannabinoid (range 0.05 to 0.67 ~g/g stool). The concentrations of metabolites were highest during the first 2 days; some stools tested positive up to the third day. In contrast, only 37% of the infants had positive results on a urine screen (fluorescent polarization immunoassay method).
2. Meconium testing was used to determine the prevalence of illicit drug abuse among pregnant women who delivered in a large perinatal center (Ostrea, E. M., Jr., Brady, M., Gause, S., Raymundo, A. L., Stevens M., Pediat.
Res. 27:251A (1990~). A total of 3010 infants were screened for the metabolites of cocaine, morphine and cannabinoids in their meconium by radioimmunoassay: 44.3% were positive for either one of the 3 drug metabolites; 41% were positive for cocaine or morphine, 30.7% were positive for cocaine (15.4% positive for cocaine only); 20.5% positive for mor-phine (7.3% positive for morphine only) and 11.5% positive for cannabinoid (5.2% positive for cannabinoid only). In S 9 2 4 ~
contrast, only 11.1% of the mothers in the entire population studied admitted to the use of drugs during pregnancy.
Rockville, MD., 1987). Although exact figures are not known, a sizable portion of drug users are women of childbearing age or are pregnant women. Infants born to these drug dependent women have multiple problems. In the neonatal period, their mortality rate is increased as well as morbidity, which includes asphyxia, prematurity, low birth weight, hyaline membrane disease, infections, aspiration pneumonia, congenital malformations, abnormal heart rate and breathing patterns and drug withdrawal (Ostrea, E. M., Chavez, C. J., J. Pediatr. 94:292-295, (1979); Zelson, C., Rubio E., and Wasserman, E., Pediatrics 48:178 (1971)). Long term sequelae are not uncommon and include delays in physical growth and mental development, -2- ~ 2 4 ~
sudden infant death syndrome, hyperactivity, ocular and neurologic abnormalities and lately, a risk to acquired immunodeficiency disease (Wilson, G. S., McCreary, M., Kean, J., and Baxter, J., Pediatrics 63:135-144 (1979);
Chavez, C. J., et al., J. Pediatrics 95:407-409 (1979);
Chasnoff, I. J., et al., Pediatrics 70:210-213 (1982);
Chavez, C. J., et al., Pediatr. Res. 12:367A, (1979); and oleske, J., et al., J. Am. Med. Assoc., 249:2345-2349 (1983)). At present, cocaine abuse among pregnant women has also become widespread and infant morbidity, notably cerebrovascular problems have been reported (Chasnoff, I.
J., et al., J. Pediatr. 108:456-459 (1986)). Because of these immediate and long term problems, infants of drug dependent mothers (IDDM) constitute a high risk group and lS have to be identified as soon as possible after birth if intervention is to be successful.
Unfortunately, the identification of the drug exposed neonate is not easy. Many of the drugs to which the fetus is exposed, in utero, do not produce immediate or recognizable effects in the neonates (Kandall, S. R., Am.
J. Dis. Child, 127:58-61 (1974)). Maternal admission of drug usage is often inaccurate because of fear of the consequences stemming from such admission. Eve~n with maternal cooperation, such information regarding the type and extent of drug usage is often inaccurate (Ostrea, E.
M., et al., J. Pediatr. 88:642-645 (1976)). One alternative is to test the infant's urine for drugs, but this procedure has its limitations since successful detection of drug metabolites in the infant's urine is dependent on time of the last drug intake by the mother or when, after birth, the infant's urine was collected. A
high rate of false negative results in neonatal urine tests can arise from the mother's abstention from the use of the drug a few days before she delivers or to the inability to obtain a sample of the infant's urine soon after birth (Halstead, A. C., et al., Clin. Biochem. 21:59-61 (1988)).
Our experience verifies this diagnostic problem. Urine ,, from 337 infants of known drug dependent mothers was tested by thin-layer chromatography. It was found that only 13%
were positive. Similarly, only 37% of the urine samples taken from drug dependent infants were positive for drugs when tested by TDX fluorescent polarization immunoassay (Ostrea, E. M., Brady, M. J., Parks, P. M., Asensio, D. C., Nalaz, A., J. Ped. 115:474-474 (1989) ). Even with more sensi~ive methods such as radioimmunoassay, 8 urine samples tested negative for drugs despite a positive test in the stools (Ostrea, E. M., ~rady, M. J., Parks, P. M., Asensio, D. C., Naluz, A., J. Ped. 115:474-474 (~1989)). Clearly, there is a need for a better way to detect prenatal drug exposure in this high risk group of infants.
A new method has been developed for identifying fetal drug exposure by detecting drug metabolites in meconium, the first green stools of the newborn infant which is passed within a few days after birth (Ostrea, E.
M., Parks, P., Brady, M., Clin. Chem. 34:2372-2373 (1989);
Ostrea, E. M., Brady, M. J., Parks, P. M., Asensio, D. C., Naluz, A., J. Ped. 115:474-474 tl989) ) . The concept behind this method was based on initial research in pregnant, morphine addicted monkeys (Ostrea, E. M., Lynn, S. N., Wayne, R. H., Stryker, J. C., Dev. Pharmacol. Ther. 9 80;
1:163-170 (1980) ) and subsequently in rats (Ostrea, E. M., Brady, M. J., Parks, P. M., Asensio, D. C., Naluz, A., J.
Ped. 115:474-477 (1989) ) which showed that a high concentration of drug metabolites were present in the gastrointestinal tract of their fetuses. we interpreted this observation to be a consequence of the following mechanism: morphine in the fetus is metabolized by the liver to water soluble glucuronide conjuga~es which are then excreted into the bile or urine (Jaffe, J., Drug addiction and drug abuse. In: Goodman, L., Gillman, A., eds. The Pharmacologic Basis of Therapeutics. London:
Collier-Macmillan, 535-584 (1989)). In either case, morphine glucuronide accumulates in the fetal intestines either from bile secretion or from fetal urine which is 206592~
swallowed via the amniotic fluid. Thus, meconium represents an excretion product which is cumulative of the entire gestation. Overall therefore, meconium acts as a reservoir of drug metabolites in the fetus; seemingly a stockpile of pharmacologic waste products throughout gestation.
Clinical studies have been conducted which have validated meconium analysis as a reliable drug screen in the newborn infant:
1. Meconium obtained from 20 infants of drug-dependent mothers and five control infants were analyzed by radioimmunoassay for the metabolites of heroin, cocaine and cannabinoids (Ostrea, E. M., Brady, M. J., Parks, P. M., Asensio, D. C., Naluz, A., J. Ped.
115-474-477 (1989)). Control stools showed no drug.
Meconium from the infants of drug-dependent mothers showed the presence of at least one drug metabolite: 80% of the infants of drug-dependent mothers showed cocaine (range 0.14 to 19.91 ~g/g stool), 55% showed morphine (range 0.41 to 14.97 ~g/g stool), and 60% showed cannabinoid (range 0.05 to 0.67 ~g/g stool). The concentrations of metabolites were highest during the first 2 days; some stools tested positive up to the third day. In contrast, only 37% of the infants had positive results on a urine screen (fluorescent polarization immunoassay method).
2. Meconium testing was used to determine the prevalence of illicit drug abuse among pregnant women who delivered in a large perinatal center (Ostrea, E. M., Jr., Brady, M., Gause, S., Raymundo, A. L., Stevens M., Pediat.
Res. 27:251A (1990~). A total of 3010 infants were screened for the metabolites of cocaine, morphine and cannabinoids in their meconium by radioimmunoassay: 44.3% were positive for either one of the 3 drug metabolites; 41% were positive for cocaine or morphine, 30.7% were positive for cocaine (15.4% positive for cocaine only); 20.5% positive for mor-phine (7.3% positive for morphine only) and 11.5% positive for cannabinoid (5.2% positive for cannabinoid only). In S 9 2 4 ~
contrast, only 11.1% of the mothers in the entire population studied admitted to the use of drugs during pregnancy.
3. The sensitivity of meconium test is high.
The method was compared to drug detection by maternal hair analysis and in depth interview of the mother (Ostrea, E.
M., Martier, S., Welch, R., Brady, M. Pediatr. Res. 27, 219A (1990); Welch, R. A., Martier, S. S., Ager, J. W., ostrea, E. M., Sokol, R. J., Substance Abuse (in press) (1990)). In 26 high risk mothers studied, the abuse of one drug during pregnancy was identiEied by history in 19 subjects (73%); by meconium analysis in 19 subjects (73.1~) and by hair analysis in 12/16 (75%) subjects. ~buse of 2 or more drugs was identified only in 6 subjects (23%) by history, as compared to 9 subjects (34.6%) by meconium analysis and in 8 (50%) by hair analysis. There was 96%
concordance of cocaine identification in hair and meconium and 73% for heroin and cannabinoids. There was also a high correlation between the cocaine concentration in meconium and in hair.
Meconium is therefore an ideal specimen for drug testing in the newborn period: (i) its collection is easy and non-invasive, (ii) it contains high concentrations of drugs and their metabolites and (ii) drugs may be present in meconium for up to the third day after birth. Meconium testing is sensitive, quantitative, and rapid. The test is therefore useful for diagnostic purposes as well as for clinical and epidemiologic research.
However, the preferred method described in copending Canadian Application No. 2,001,229, is different for mass drug screening of meconium in infants since the former involve separate extractions for the different drugs with acidified water or methanol and analysis by immunoassay, particularly radioimmunoassay. It is desirable to modify the procedure to provide for mass screening and particularly to allow analysis by other methods such as enzyme immunoassay 206S~24 (EMIT), fluorescent polarization method, HPLC and gas chromatography/mass spectroscopy.
OBJECTS
It is therefore an object of the present invention to provide an improved method for testing for drug metabolites in infants which allows for rapid mass screening. It is further an object of the present invention to provide other methods of detection of drugs which are also reliable. Further still, it is an object of the present invention to provide an improved method which is relatively simple and economical to perform. These and other objects will become increasingly apparent by reference to the following description.
GENERAL DESCRIPTION
The present invention relates to a method for detecting maternally transferred drug metabolites in a newborn infant which comprises: isolating meconium from the newborn infant which possibly contains the transferred drug metabolites from the mother; extracting the drug metabolites from the meconium in an aqueous solution containing methanol in an amount less than about 30% by volume with a buffered pH between about 6 and 7 and assaying the solution for the drug metabolites, preferably using enzyme immunoassay (EMIT), fluorescent polarization method (TDX) and gas chromatography/mass spectroscopy.
Preferably the methanol represents about 10 to 30 percent by volume of the aqueous solution. The buffered aqueous methanol eliminates cross-reactivity or interference secondary to the extraction of unwanted compounds from the meconium.
The drug metabolites are preferably extracted from the meconium using a solution of 0.1 M phosphate buffered methanol (4 parts volume 0.1 M phosphate buffer tpH = 6.4-6.8] and l part volume methanol). This mixture allows a one-step complete separation of all of the drug metabolites in meconium and the exclusion of other compounds in meconium which can cross-react in the 2 ~ 4 subsequent analytical detection assays. This method is thus an improvement over the 2referred two-step procedure described in copending Canadian Application 2,001,229.
The buffered methanol solution used ~or the optimum extraction of the drug metabolites from the meconium has a pH between about 6 and 7. A buffer, such as 0.lM phosphate buffer, is used to maintain the pH. The preferred buffer is a mixture of sodium or potassium monoQhosphate and biphosphate.
The buffered methanol extract is further cleared of particulate matter by centrifugation using micropartition centrifuge tubes.
Once the drug metabolites are extracted from the meconium and filtered, standard assays are performed in order to detect the presence of the drug metabolites.
These assays can be radioimmunoassays, enzyme immunoassay (ELISA or EMIT) using antibodies or appropriate probes which are specific for the drug metabolites. The antibody or multiple antibody sandwich assays is well known to those skilled in the art. Fluorescent polarization (TDX) assays and gas chromatography/mass spectroscopy can also be used to identify the metabolites. Further still, other quantitative or qualitative chemical tests can be used to assay for the drug metabolites in the isolated solution as is well known to those skilled in the art.
SPECIFIC DESCRIPTION
METHODS
Meconium was collected from infants some of whom were born to mothers who by history had abused drugs during pregnancy, commonly heroin, cocaine, methadone, cannabinoids, amphetamines, barbiturates and benzodiazepines. The stools were obtained directly from the diaper.
~?
RESULTS
Example 1 The method of this Example involves a one-step drug extraction using buffered methanol and analysis by enzyme immunoassay (EMIT) or fluorescent polarization method (TDX) or radioimmunoassay.
The steps in the method are:
1. Measure 0.2 to 0.5 g of meconium and suspend in 2 to 5 ml of 0.1 M phosphate buffered methanol (4:1 v/v aqueous buffered solution to methanol, pH = 6.4 to 6.8).
2. Centrifuge at 2000 rpm for 10 minutes.
3. Transfer supernate to Amicon Centrifree~
(American Division, W. R. Grace and Co., Danvers, MA) micropartition tubes and centrifuge at 2100 rpm for 30 minutes.
The method was compared to drug detection by maternal hair analysis and in depth interview of the mother (Ostrea, E.
M., Martier, S., Welch, R., Brady, M. Pediatr. Res. 27, 219A (1990); Welch, R. A., Martier, S. S., Ager, J. W., ostrea, E. M., Sokol, R. J., Substance Abuse (in press) (1990)). In 26 high risk mothers studied, the abuse of one drug during pregnancy was identiEied by history in 19 subjects (73%); by meconium analysis in 19 subjects (73.1~) and by hair analysis in 12/16 (75%) subjects. ~buse of 2 or more drugs was identified only in 6 subjects (23%) by history, as compared to 9 subjects (34.6%) by meconium analysis and in 8 (50%) by hair analysis. There was 96%
concordance of cocaine identification in hair and meconium and 73% for heroin and cannabinoids. There was also a high correlation between the cocaine concentration in meconium and in hair.
Meconium is therefore an ideal specimen for drug testing in the newborn period: (i) its collection is easy and non-invasive, (ii) it contains high concentrations of drugs and their metabolites and (ii) drugs may be present in meconium for up to the third day after birth. Meconium testing is sensitive, quantitative, and rapid. The test is therefore useful for diagnostic purposes as well as for clinical and epidemiologic research.
However, the preferred method described in copending Canadian Application No. 2,001,229, is different for mass drug screening of meconium in infants since the former involve separate extractions for the different drugs with acidified water or methanol and analysis by immunoassay, particularly radioimmunoassay. It is desirable to modify the procedure to provide for mass screening and particularly to allow analysis by other methods such as enzyme immunoassay 206S~24 (EMIT), fluorescent polarization method, HPLC and gas chromatography/mass spectroscopy.
OBJECTS
It is therefore an object of the present invention to provide an improved method for testing for drug metabolites in infants which allows for rapid mass screening. It is further an object of the present invention to provide other methods of detection of drugs which are also reliable. Further still, it is an object of the present invention to provide an improved method which is relatively simple and economical to perform. These and other objects will become increasingly apparent by reference to the following description.
GENERAL DESCRIPTION
The present invention relates to a method for detecting maternally transferred drug metabolites in a newborn infant which comprises: isolating meconium from the newborn infant which possibly contains the transferred drug metabolites from the mother; extracting the drug metabolites from the meconium in an aqueous solution containing methanol in an amount less than about 30% by volume with a buffered pH between about 6 and 7 and assaying the solution for the drug metabolites, preferably using enzyme immunoassay (EMIT), fluorescent polarization method (TDX) and gas chromatography/mass spectroscopy.
Preferably the methanol represents about 10 to 30 percent by volume of the aqueous solution. The buffered aqueous methanol eliminates cross-reactivity or interference secondary to the extraction of unwanted compounds from the meconium.
The drug metabolites are preferably extracted from the meconium using a solution of 0.1 M phosphate buffered methanol (4 parts volume 0.1 M phosphate buffer tpH = 6.4-6.8] and l part volume methanol). This mixture allows a one-step complete separation of all of the drug metabolites in meconium and the exclusion of other compounds in meconium which can cross-react in the 2 ~ 4 subsequent analytical detection assays. This method is thus an improvement over the 2referred two-step procedure described in copending Canadian Application 2,001,229.
The buffered methanol solution used ~or the optimum extraction of the drug metabolites from the meconium has a pH between about 6 and 7. A buffer, such as 0.lM phosphate buffer, is used to maintain the pH. The preferred buffer is a mixture of sodium or potassium monoQhosphate and biphosphate.
The buffered methanol extract is further cleared of particulate matter by centrifugation using micropartition centrifuge tubes.
Once the drug metabolites are extracted from the meconium and filtered, standard assays are performed in order to detect the presence of the drug metabolites.
These assays can be radioimmunoassays, enzyme immunoassay (ELISA or EMIT) using antibodies or appropriate probes which are specific for the drug metabolites. The antibody or multiple antibody sandwich assays is well known to those skilled in the art. Fluorescent polarization (TDX) assays and gas chromatography/mass spectroscopy can also be used to identify the metabolites. Further still, other quantitative or qualitative chemical tests can be used to assay for the drug metabolites in the isolated solution as is well known to those skilled in the art.
SPECIFIC DESCRIPTION
METHODS
Meconium was collected from infants some of whom were born to mothers who by history had abused drugs during pregnancy, commonly heroin, cocaine, methadone, cannabinoids, amphetamines, barbiturates and benzodiazepines. The stools were obtained directly from the diaper.
~?
RESULTS
Example 1 The method of this Example involves a one-step drug extraction using buffered methanol and analysis by enzyme immunoassay (EMIT) or fluorescent polarization method (TDX) or radioimmunoassay.
The steps in the method are:
1. Measure 0.2 to 0.5 g of meconium and suspend in 2 to 5 ml of 0.1 M phosphate buffered methanol (4:1 v/v aqueous buffered solution to methanol, pH = 6.4 to 6.8).
2. Centrifuge at 2000 rpm for 10 minutes.
3. Transfer supernate to Amicon Centrifree~
(American Division, W. R. Grace and Co., Danvers, MA) micropartition tubes and centrifuge at 2100 rpm for 30 minutes.
4. Obtain aliquots of the filtrate and analyze in duplicate for cocaine, opiates, cannabinoids and/or methamphetamine by enzyme immunoassay (EMIT - Sylva Co., Palo Alto, CA) or fluorescent polarization method (TDX, Abbott Laboratories Diagnostics Div., Irving, TX).
The minimum concentration values for testing found using these methods were: cannabinoid 50 ng/ml;
cocaine 50 ng/ml; opiate 60 ng/ml; methamphetamine 50 ng/ml, which are acceptable for most purposes.
The accuracy of the modified method was tested by comparing the results of simultaneous analysis of 61 meconium samples for cocaine, opiate and cannabinoid metabolites by the original method (described in the Examples of copending Canadian Application No. 2,001,229) using a radioimmunoassay and the improved method is shown in Tables I-III).
~'~
Table I. Comparison of Morphine Detection by the Original and Modified Methods(l):
Original Method Modified Negative Positive Total 5Method Negative 52 0 52 Positive 1 8 9 Total 53 8 61 Sensitivity = 8/8 (100%) Specificity = 52/53 (98%) + Predictive value 8/9 = 89%
- Predictive value 52/52 = 100%
(l)The original method is treated as the "gold" standard by which the improved method is judged.
Table II. Comparison of Cocaine Detection by the Original and Modified Methods:
: Original Method Modified Negative Positive Total Method Negative 21 1 22 Positive 1 38 39 Total 22 39 61 Sensitivity = 38/39 (98%) Specificity = 21/22 (95%) + Predictive value 38/39 (97%) - Predictive value 21/22 = (95%) 20~924 Table III. Comparison of Cannabinoid Detection by the Original and Modified Methods:
Original Method Modified Negative Positive Total Method Negative 39 1 40 Positive 0 0 0 Total 39 1 40 In the 61 samples analyzed, opiates were detected in 8 (13%) by the original method and in 9 (15%) by the modified method; cocaine was detected in 39 (64%) by the original method and in 39 (64%) by the modified method. The sensitivity and specificity of the modified method for opiate detection was 100~ and 98%, respectively (positive and negative predictive values of 89% and 100~, respectively); for detecting cocaine, sensitivity and specificity of 98% and 95%, respectively (positive and negative predictive values of 97~ and 95%, respectively.
Forty samples were available for analysis for cannabinoids;
40 were found to be negative by the modified method; 39 were negative and 1 positive by the original method.
It was concluded that the improved method for meconium testing was useful for mass drug screening in the newborn infant. The method is easy, rapid and highly sensitive and specific for the drugs analyzed. Likewise, adaptation of the test to enzyme immunoassay (rather than radioimmunoassay) makes it practical for clinical laboratory use.
Example 2 Until recently, various immunoassays have been the only analytical methods used to analyze meconium for drugs. GC/MS (GC/mass spectroscopy) was adapted to meconium testing. This provides for the definitive - ~n~5s~
identification of drugs in meconium, as well as precise information on the types of drug metabolite present. This Example 2 shows GC/MS analysis of meconium for cocaine.
The steps o~ the method are:
1. Obtain 0.5 to 1.O g of meconium and suspend in 5 to 10 ml of 0.1 M Phosphate buffered methanol (4:1 v/v aqueous buffered solution to methanol, pH = 6.4 to 6.8).
2. Centrifuge at 2000 rpm for 10 minutes.
3. Transfer supernate to ~micon Centrifree~
micropartition tubes and centrifuge at 2100 rpm for 30 minutes.
4. Recover filtrate and subject to solid phase extraction using a Bond-Elute column (Analytichem Intl., Harbor City, CA) utilizing the protocol for cocaine.
The minimum concentration values for testing found using these methods were: cannabinoid 50 ng/ml;
cocaine 50 ng/ml; opiate 60 ng/ml; methamphetamine 50 ng/ml, which are acceptable for most purposes.
The accuracy of the modified method was tested by comparing the results of simultaneous analysis of 61 meconium samples for cocaine, opiate and cannabinoid metabolites by the original method (described in the Examples of copending Canadian Application No. 2,001,229) using a radioimmunoassay and the improved method is shown in Tables I-III).
~'~
Table I. Comparison of Morphine Detection by the Original and Modified Methods(l):
Original Method Modified Negative Positive Total 5Method Negative 52 0 52 Positive 1 8 9 Total 53 8 61 Sensitivity = 8/8 (100%) Specificity = 52/53 (98%) + Predictive value 8/9 = 89%
- Predictive value 52/52 = 100%
(l)The original method is treated as the "gold" standard by which the improved method is judged.
Table II. Comparison of Cocaine Detection by the Original and Modified Methods:
: Original Method Modified Negative Positive Total Method Negative 21 1 22 Positive 1 38 39 Total 22 39 61 Sensitivity = 38/39 (98%) Specificity = 21/22 (95%) + Predictive value 38/39 (97%) - Predictive value 21/22 = (95%) 20~924 Table III. Comparison of Cannabinoid Detection by the Original and Modified Methods:
Original Method Modified Negative Positive Total Method Negative 39 1 40 Positive 0 0 0 Total 39 1 40 In the 61 samples analyzed, opiates were detected in 8 (13%) by the original method and in 9 (15%) by the modified method; cocaine was detected in 39 (64%) by the original method and in 39 (64%) by the modified method. The sensitivity and specificity of the modified method for opiate detection was 100~ and 98%, respectively (positive and negative predictive values of 89% and 100~, respectively); for detecting cocaine, sensitivity and specificity of 98% and 95%, respectively (positive and negative predictive values of 97~ and 95%, respectively.
Forty samples were available for analysis for cannabinoids;
40 were found to be negative by the modified method; 39 were negative and 1 positive by the original method.
It was concluded that the improved method for meconium testing was useful for mass drug screening in the newborn infant. The method is easy, rapid and highly sensitive and specific for the drugs analyzed. Likewise, adaptation of the test to enzyme immunoassay (rather than radioimmunoassay) makes it practical for clinical laboratory use.
Example 2 Until recently, various immunoassays have been the only analytical methods used to analyze meconium for drugs. GC/MS (GC/mass spectroscopy) was adapted to meconium testing. This provides for the definitive - ~n~5s~
identification of drugs in meconium, as well as precise information on the types of drug metabolite present. This Example 2 shows GC/MS analysis of meconium for cocaine.
The steps o~ the method are:
1. Obtain 0.5 to 1.O g of meconium and suspend in 5 to 10 ml of 0.1 M Phosphate buffered methanol (4:1 v/v aqueous buffered solution to methanol, pH = 6.4 to 6.8).
2. Centrifuge at 2000 rpm for 10 minutes.
3. Transfer supernate to ~micon Centrifree~
micropartition tubes and centrifuge at 2100 rpm for 30 minutes.
4. Recover filtrate and subject to solid phase extraction using a Bond-Elute column (Analytichem Intl., Harbor City, CA) utilizing the protocol for cocaine.
5. Treat the purified residue with BSTFA
(N,O-bis-trimethylsilyl-trifluoroacetamide) to form the trimethylsilyl derivatives and ~ inject into a Finnigan ITD BC/MS (Finnigan Corp., San Jose, CA).
(N,O-bis-trimethylsilyl-trifluoroacetamide) to form the trimethylsilyl derivatives and ~ inject into a Finnigan ITD BC/MS (Finnigan Corp., San Jose, CA).
6. Cocaine and benzoylecgonine mass spectra are identified through their characteristic ion masses (cocaine - m/z 82, 105, 182, 303;
benzoylecgonine = m/z 82, 105, 240, 361.
RESULTS: Eight meconium samples, all positive for cocaine by enzyme (EMIT) and radioimmunoassays per the method described in the Examples of copending Canadian Application No. 2,001,229 (at cutoff concentration of 50 ng/ml) were analyzed by GC/MS according to the above method. Cocaine or its metabolites, benzoylecgonine were detected in the samples analyzed by GC/MS: 6/9 (65%) showed the parent compound, cocaine and 7/9 (78%) showed benzoylecgonine (Table IV).
., . . ~.
206~24 Table IV. Distribution of cocaine and benzoylecgonine.
GC/MS Results for Meconium Sample # BE Cocaine + +
2 +
3 + +
4 + +
S + +
+
benzoylecgonine = m/z 82, 105, 240, 361.
RESULTS: Eight meconium samples, all positive for cocaine by enzyme (EMIT) and radioimmunoassays per the method described in the Examples of copending Canadian Application No. 2,001,229 (at cutoff concentration of 50 ng/ml) were analyzed by GC/MS according to the above method. Cocaine or its metabolites, benzoylecgonine were detected in the samples analyzed by GC/MS: 6/9 (65%) showed the parent compound, cocaine and 7/9 (78%) showed benzoylecgonine (Table IV).
., . . ~.
206~24 Table IV. Distribution of cocaine and benzoylecgonine.
GC/MS Results for Meconium Sample # BE Cocaine + +
2 +
3 + +
4 + +
S + +
+
7 - +
8 +
9 -- +
Total 7/9 t78~) 6/9 (67%~
It will be appreciated that the foregoing description is only illustrative of the present invention and that this invention is limited only by the hereinafter appended claims.
Total 7/9 t78~) 6/9 (67%~
It will be appreciated that the foregoing description is only illustrative of the present invention and that this invention is limited only by the hereinafter appended claims.
Claims (16)
1. A method for detecting maternally transferred drug metabolites in a newborn infant which comprises:
(a) isolating meconium from the newborn infant which possibly contains the transferred drug metabolites from the mother;
(b) extracting the drug metabolites from the meconium in an aqueous solution containing methanol in an amount of less than about 30 % by volume with a buffered pH between about 6 and 7; and (c) assaying the solution for the drug metabolites.
(a) isolating meconium from the newborn infant which possibly contains the transferred drug metabolites from the mother;
(b) extracting the drug metabolites from the meconium in an aqueous solution containing methanol in an amount of less than about 30 % by volume with a buffered pH between about 6 and 7; and (c) assaying the solution for the drug metabolites.
2. The method of Claim 1 wherein solids present in the meconium are removed by centrifugation from the solution.
3. The method of Claim 1 wherein the solution is buffered with a phosphate to a pH between about 6 and 7.
4. The method of Claim 3 wherein the concentration of phosphate buffer is 0.1M.
5. The method of Claim 1 wherein the drug metabolites are selected from the group consisting of cocaine, morphine, cannabinoids and methamphetamine metabolites.
6. The method of Claim 1 wherein the infant is human and the meconium is fecal.
7. The method of Claim 1 wherein the assay is an immunoassay.
8. The method of Claim 7 wherein the assay is an enzyme linked immunoassay.
9. The method of Claim 7 wherein the assay is a radioimmunoassay.
10. The method of Claim 1 wherein the assay is by fluorescent polarization.
11. The method of Claim 1 wherein the assay is by gas chromatography.
12. The method of Claim 11 wherein in addition as a control the solution is assayed by mass spectroscopy which identifies peaks uniquely produced by the drug metabolites.
13. The method of Claim 12 wherein, prior to assaying, the metabolites in the solution are reacted with N,O-bis-trimethylsilyl-trifluoroacetamide to form trimethylsilyl derivatives of the metabolites.
14. The method of Claim 1 wherein, as a control, the solution is assayed by mass spectroscopy which identifies peaks uniquely produced by the drug metabolites.
15. The method of Claim 14 wherein the metabolites in the solution are reacted with N,O-bis-trimethylsilyl-trifluoroacetamide to form trimethylsilyl derivatives of the metabolites.
16. The method of Claim 1 wherein the drug metabolites are selected from the group consisting of cocaine, morphine, cannabinoid and amphetamine metabolites.
Applications Claiming Priority (2)
| Application Number | Priority Date | Filing Date | Title |
|---|---|---|---|
| US691,994 | 1991-04-26 | ||
| US07/691,994 US5185267A (en) | 1988-10-28 | 1991-04-26 | Method for detecting maternally transferred drug metabolites in newborn infants |
Publications (2)
| Publication Number | Publication Date |
|---|---|
| CA2065924A1 CA2065924A1 (en) | 1992-10-27 |
| CA2065924C true CA2065924C (en) | 1998-08-11 |
Family
ID=24778842
Family Applications (1)
| Application Number | Title | Priority Date | Filing Date |
|---|---|---|---|
| CA 2065924 Expired - Fee Related CA2065924C (en) | 1991-04-26 | 1992-04-13 | Method for detecting maternally transferred drug metabolites in newborn infants |
Country Status (1)
| Country | Link |
|---|---|
| CA (1) | CA2065924C (en) |
-
1992
- 1992-04-13 CA CA 2065924 patent/CA2065924C/en not_active Expired - Fee Related
Also Published As
| Publication number | Publication date |
|---|---|
| CA2065924A1 (en) | 1992-10-27 |
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