US20050048499A1 - Tandem mass spectrometry method for the genetic screening of inborn errors of metabolism in newborns - Google Patents

Tandem mass spectrometry method for the genetic screening of inborn errors of metabolism in newborns Download PDF

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US20050048499A1
US20050048499A1 US10/652,732 US65273203A US2005048499A1 US 20050048499 A1 US20050048499 A1 US 20050048499A1 US 65273203 A US65273203 A US 65273203A US 2005048499 A1 US2005048499 A1 US 2005048499A1
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Blas Cerda
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PerkinElmer Health Sciences Inc
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Assigned to PERKINELMER LIFE SCIENCES, INC. reassignment PERKINELMER LIFE SCIENCES, INC. ASSIGNMENT OF ASSIGNORS INTEREST (SEE DOCUMENT FOR DETAILS). Assignors: CERDA, BLAS A.
Priority to PCT/US2004/028238 priority patent/WO2005021779A1/en
Priority to JP2006524947A priority patent/JP4838129B2/ja
Priority to AU2004269410A priority patent/AU2004269410B2/en
Priority to ES04782672.2T priority patent/ES2527306T3/es
Priority to US10/539,273 priority patent/US20060234326A1/en
Priority to EP04782672.2A priority patent/EP1664325B1/en
Priority to CA2537034A priority patent/CA2537034C/en
Publication of US20050048499A1 publication Critical patent/US20050048499A1/en
Assigned to PERKINELMER LAS, INC. reassignment PERKINELMER LAS, INC. CHANGE OF NAME (SEE DOCUMENT FOR DETAILS). Assignors: PERKINELMER LIFE SCIENCES, INC.
Priority to US12/349,669 priority patent/US8318417B2/en
Priority to JP2011126859A priority patent/JP2011167208A/ja
Priority to US13/357,324 priority patent/US8399186B2/en
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    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12QMEASURING OR TESTING PROCESSES INVOLVING ENZYMES, NUCLEIC ACIDS OR MICROORGANISMS; COMPOSITIONS OR TEST PAPERS THEREFOR; PROCESSES OF PREPARING SUCH COMPOSITIONS; CONDITION-RESPONSIVE CONTROL IN MICROBIOLOGICAL OR ENZYMOLOGICAL PROCESSES
    • C12Q1/00Measuring or testing processes involving enzymes, nucleic acids or microorganisms; Compositions therefor; Processes of preparing such compositions
    • GPHYSICS
    • G01MEASURING; TESTING
    • G01NINVESTIGATING OR ANALYSING MATERIALS BY DETERMINING THEIR CHEMICAL OR PHYSICAL PROPERTIES
    • G01N33/00Investigating or analysing materials by specific methods not covered by groups G01N1/00 - G01N31/00
    • G01N33/48Biological material, e.g. blood, urine; Haemocytometers
    • G01N33/50Chemical analysis of biological material, e.g. blood, urine; Testing involving biospecific ligand binding methods; Immunological testing
    • G01N33/68Chemical analysis of biological material, e.g. blood, urine; Testing involving biospecific ligand binding methods; Immunological testing involving proteins, peptides or amino acids
    • G01N33/6893Chemical analysis of biological material, e.g. blood, urine; Testing involving biospecific ligand binding methods; Immunological testing involving proteins, peptides or amino acids related to diseases not provided for elsewhere
    • GPHYSICS
    • G01MEASURING; TESTING
    • G01NINVESTIGATING OR ANALYSING MATERIALS BY DETERMINING THEIR CHEMICAL OR PHYSICAL PROPERTIES
    • G01N2800/00Detection or diagnosis of diseases
    • G01N2800/04Endocrine or metabolic disorders

Definitions

  • the present invention is in the field of spectroscopy. Specifically, the present invention is related to methods for use with mass spectrometry.
  • IEM Inborn errors of metabolism
  • the lack or inactivity of key enzymes due to IEM can result in the accumulation of precursor metabolites, the accumulation of secondary product metabolites, and/or the lack of primary product metabolites.
  • the overriding result of genetic mutations in IEM is the lack or inactivity of essential enzymes.
  • the first is to measure the amounts of marker metabolites, i.e. measure the accumulation of the precursor or alternate product metabolites and/or measure the decrease of the primary product metabolite.
  • the second possibility is to measure the enzyme activity of the unknown patient sample.
  • the first approach is generally performed by tandem mass spectrometry (MS/MS) methods.
  • MS/MS tandem mass spectrometry
  • a small disc from a patient sample in the form of a blood spot dried on filter paper is punched into a microtiter plate well.
  • a solvent containing a set of internal standards is added to each well containing a blood spot punch to extract the marker metabolites from the sample.
  • the solution containing the extracted metabolites and internal standards is then transferred to a new microtiter plate and the solution is dried under heated nitrogen.
  • a new solution containing acid and butanol is added to create butyl ester derivatives of the extracted metabolites.
  • the derivatized sample is then dried under heated nitrogen again to remove the excess derivatizing agent and reconstituted with a third solvent type. Finally, the concentration of the desired metabolites is then measured by isotope dilution MS/MS. This approach is used for measuring the concentrations of acylcarnitines and amino acids (such as shown in U.S. Pat. Nos. 6,258,605 B1 and 6,455,321 B1 to Chace; hereby incorporated herein by reference). Below is a full protocol for such MS/MS method for the analysis of amino acids and acylcarnitines:
  • the second possibility, to measure enzyme activity is generally performed by punching a small disc of a blood spot sample into a microtiter well. Subsequently, a solution containing buffers is added to reconstitute an enzyme of interest. Once the enzyme is reconstituted, a second solution containing a fluorescent analog to the natural substrate is added and the sample is incubated for a predetermined amount of time to allow the reconstituted enzyme to act on the artificial substrate. Once sufficient time has elapsed, a third type of solvent is added to stop the reaction (precipitate.the enzyme). The plate containing the sample is then placed in a fluorometer and the fluorescence of the artificial product is measured. The fluorescence can then be correlated to a particular level of enzyme activity. 4-5
  • MS/MS approach allows for the simultaneous analysis of several metabolite markers (acylcarnitines and amino acids) from a single sample and it alleviates environmental factors that affect enzyme activity such as exposure to light, temperature ranges, and humidity.
  • metabolite markers acylcarnitines and amino acids
  • the disadvantages are that the sample preparation is lengthy and complicated as well as that it employs harmful solvents such as butanol in HCI that can be very deleterious to personnel and equipment. Additionally and more importantly, is the fact that certain IEM cannot be screened for by MS/MS because the marker metabolites have many natural isomers also present in blood that prevent the measurement of their concentration.
  • a case in point is galactose metabolism in which the measurement of the marker galactose-1-phosphate is impeded because several other phosphorylated sugars present in blood such as glucose-1-phospahate are isomeric with galactose-1-phosphate.
  • the levels of potential metabolite markers are too low in blood to be measured effectively by MS/MS at a stage in which the affected individual still does not show any symptoms. In these cases MS/MS would only be able to detect the marker metabolites at a clinical stage that may be too late to administer effective preventive treatment.
  • Measuring enzyme activity by fluorometry alleviates some of the disadvantages suffered by MS/MS.
  • isomeric interferences there is no better discriminator of isomers than the natural enzymes.
  • Enzymes have great specificity for their natural substrates such that isomeric interferences are generally not an issue.
  • the levels of markers are too low to be measured directly by MS/MS, one can reconstitute the enzyme of interest and add enough artificial substrate to drive the reaction and be able to discriminate patients with normal versus decreased enzyme activity.
  • the disadvantages of fluorometric methods are that one has to employ artificial substrates that are tagged with a fluorescent group.
  • the substrates are different enough from their natural counter parts that enzyme activity using such substrates is inherently reduced and thus the sensitivity of the assays. Additionally, because one estimates enzyme activity by measuring fluorescence it is not practical to fully take advantage of multiplex analysis. In some cases, tags that would fluoresce at different wavelengths can be used, but instruments capable of reading multiple fluorescent labels can only handle a few of such markers. Because of this, most enzyme activity assays employing some type of light emission for measurement are single analyte assays.
  • the present invention provides methods for simultaneous measurement of enzyme activity and relatively polar and/or relatively non-polar analyte concentration, thereby overcoming the deficiencies of prior art methodologies. More specifically, the present invention does not require sample derivatization or substrate tagging with fluorescent groups. The present invention measurement of enzyme activity and metabolite elution may be performed in the same mixture, followed by tandem mass spectrometry assay.
  • the present invention is a method for genetic screening of inborn errors of metabolism in a newborn by tandem mass spectrometry, the method comprising the steps of: (a) obtaining a dried blood sample containing at least one enzyme, at least one relatively polar metabolic analyte, and at least one relatively non-polar metabolic analyte; (b) adding a solution of a relatively polar solvent to the dried blood sample so as to reconstitute the at least one enzyme in the dried blood sample and so as to extract the at least one relatively polar analyte therefrom, thereby forming a first solution; (c) incubating the first solution with a substrate for the at least one enzyme so as to create an enzymatic product; (d) adding a solution of a relatively non-polar solvent (this solution may contain acid at the required concentration to precipitate the enzyme) to the first solution so as to stop the reaction of the at least one enzyme and so as to extract the at least one relatively non-polar analyte, so as to form a second solution;
  • the solution of a relatively polar solvent additionally may also comprise at least one component selected from the group consisting of: an internal standard for the at least one relatively polar analyte, an internal standard(s) for the enzymatic product(s) to be measured, an internal standard for the at least one relatively non-polar analyte, one or more substrates for the enzyme(s), and a buffer.
  • an internal standard for the at least one relatively polar analyte an internal standard(s) for the enzymatic product(s) to be measured
  • an internal standard for the at least one relatively non-polar analyte one or more substrates for the enzyme(s)
  • a buffer one or more substrates for the enzyme(s)
  • the solution of a relatively non-polar solvent may additionally comprise at least one component selected from the group consisting of: an internal standard for at least one relatively polar analyte, an internal standard(s) for the enzymatic product(s) to be measured, an internal standard for at least one relatively non-polar analyte, and a buffer. These internal standard components may be labeled.
  • the present invention may be applied to a method for genetic screening of inborn errors of metabolism in a newborn by tandem mass spectrometry.
  • the method comprises placing a blood spot from the newborn into a microtiter plate well.
  • a solution of a polar solvent is then added to the well so as to reconstitute enzymes in the blood spot and to extract polar analytes, thereby forming a sample.
  • the sample is then incubated for a predetermined period of time to extract metabolites and to allow substrate to product conversion by the reconstituted enzyme(s).
  • a second solution is then added to the sample to stop enzymatic reactions. At this point the sample is mixed for a predetermined period of time (optional step) to allow additional metabolite extraction.
  • the sample is then measured by tandem mass spectrometry so as to identify analyte concentration and enzyme activity. The analyte concentration and enzyme activity are then used to determine whether the newborn is affected by any inborn errors of metabolism.
  • the term “metabolite ” shall mean (1) a substance produced by metabolism; (2) a substance necessary for or taking part in a particular metabolic process; (3) a product of metabolism; (4) a substance produced by metabolic action, as urea; or (5) any substance involved in metabolism (either as a product of metabolism or as necessary for metabolism).
  • labeled shall include isotopic labeling, fluorescent labeling, and other forms of chemical labeling as are known to those of ordinary skill in the art.
  • the solution of polar solvent comprises at least one component selected from the group consisting of: an internal standard for an analyte, an internal standard for an enzymatic product to be measured, a substrate, and a buffer. It is most preferred that at least one of the at least one components are labeled.
  • the internal standard(s) may be one or more internal standards for each class of analyte, or even one internal standard per analyte.
  • the analyte(s) may then be compared to the internal standard(s).
  • the second solution is less-polar than the solution of polar solvent. It is preferred that the second solution comprises at least one component selected from the group consisting of: an internal standard for an analyte, an internal standard for an enzymatic product to be measured, and a buffer. It is most preferred that at least one of the at least one component is labeled.
  • the method may additionally comprise the step of adding at least one detergent to the sample prior to mixing.
  • a second method for the genetic screening of inborn errors of metabolism in a newborn by tandem mass spectrometry of the present invention comprises placing a blood spot sample from the newborn into a microtiter plate well so as to form a sample.
  • the microtiter plate well is treated with at least one pre-treater selected from the group consisting of: an internal standard for the at least one relatively polar analyte, an internal standard(s) for the enzymatic product(s) to be measured, an internal standard for the at least one relatively non-polar analyte, one or more substrates for the enzyme(s), and a buffer.
  • These internal standard components may be labeled.
  • These pre-treaters are dry-coated onto the microtiter well.
  • the method may additionally comprise the step of adding a polar solvent to the well after placing the blood spot therein. Additionally, the method may comprise adding a solution after incubation so as to stop enzymatic reactions. Optionally, the method may comprise mixing the sample for a predetermined period of time.
  • Tandem mass spectrometry is used to determine analyte concentration and enzyme activity.
  • the analyte concentration and enzyme activity data are used to determine whether the newborn is affected by any inborn errors of metabolism.
  • the present invention includes both a combined metabolite and enzyme activity sample preparation method, with a single tandem mass spectrometry analysis in which the internal standards and substrates are incorporated within the solvents or are already present on the microtiter well as dry-coated materials.
  • the present invention consolidates the measurements of enzyme activity and metabolite concentration measurement into a single assay that does not require sample derivatization.
  • the present invention thus represents an improvement over current newborn screening methodologies that are performed independently from each other.
  • Some of the many applications for the methods of the present invention include but are not limited to assays for biotinidase deficiency, assays pertaining to disorders in carbohydrate metabolism (such as galactosemia), assays for lyposomal storage disorders (such as mucopolysaccharidoses, sphingolipodoses, oligosaccharidoses and mucolipidoses), fatty acid ⁇ -oxidation and organic acid metabolic disorders, amino acid metabolism disorders, and congenital adrenal hyperplasia.
  • Other substances that may be determined from the methods of the present invention include but are not limited to carbohydrates, bile acids, very long chain fatty acids and steroids.
  • FIG. 1 is a schematic of a newborn screening method for metabolite concentration measurement by MS/MS in accordance with the prior art.
  • FIG. 2 is a schematic of a newborn screening method for enzyme activity measurement by fluorometry in accordance to prior art.
  • FIG. 3 is a schematic of a newborn screening method for combined enzyme activity and metabolite concentration measurement by MS/MS in accordance with one embodiment of the present invention.
  • FIG. 4 is a schematic of a newborn screening method for combined enzyme activity and metabolite concentration measurement by MS/MS in accordance with another embodiment of the present invention.
  • MS/MS methods require sample derivatization.
  • the conditions required to carry out this chemical modification of the sample may destroy both the enzymatic products as well as the enzymes; thus it may be impossible to measure enzyme activity with the current MS/MS methods.
  • many of the natural substrates and/or products involved in the metabolic pathways currently probed by enzyme activity assays belong to complex isomeric classes and/or are present in very low concentration or in conjugated forms. Therefore, it is not practical with the current MS/MS newborn screening methodology to accurately measure their concentration. Transforming these enzyme activity assays into MS/MS metabolite concentration assays is thus currently impractical.
  • the present invention provides a method that does not require sample derivatization or substrate tagging with fluorescent groups and that consolidates the two types of assays into a single sample preparation.
  • the invention is a very simple and easy to use comprehensive clinical method.
  • a blood spot from a newborn is placed into microtiter plate wells (any plate format).
  • this solution can contain internal standards for the enzymatic products to be measured.
  • This step accomplishes two tasks: a) enzyme reconstitution and b) extraction of all polar analytes present in the sample. Buffers can also be added if necessary.
  • the internal standards are analogs of the analytes (preferably, but not required, isotopically labeled analogs). A multitude of standards can be added (whichever are desired). The internal standards can also include (isotopically or other wise labeled) analogs of the enzymatic products.
  • the substrates (whichever needed) do not need to be tagged with fluorescent groups; they can be isotopically or other wise labeled analogs to the natural substrate so that they have more physiologic affinity to their corresponding enzyme. In this case, the labels are different than in the enzymatic product internal standard to avoid confusion.
  • the solution in this step is polar (for instance, any solvent varying from pure water to any mixture of polar solvents and buffers).
  • polar for instance, any solvent varying from pure water to any mixture of polar solvents and buffers.
  • the sample is incubated for a predetermined amount of time. During this time, the reconstituted enzymes are acting on the specific added substrates and the metabolites are being extracted simultaneously.
  • this solvent can also contain a multitude of non-polar (less polar) internal standards (including internal standards for the products of the enzymatic reactions). For example, if we add methanol at this step, enzymes will denature while at the same time we can extract less polar analytes such as acylcarnitines, bile acids, fatty acids, less polar amino acids, organic acids, etc. The solution in this step is less polar than the polar solution previously added. At some point (depending on polarity differences), the two solutions may not be miscible with each other. In these instances, detergents can be added to homogenize the solutions.
  • the sample is measured by tandem mass spectrometry using isotope dilution MS/MS.
  • Analyte concentration is measured by comparing intensities of the analytes against the intensities of the corresponding internal standards of known concentration.
  • Enzyme activity is measured by determining the concentration of the labeled product.
  • the concentration of the labeled product is measured by comparing the intensity of the product against the intensity of the corresponding internal standard of known concentration.
  • the concentration of the enzymatic product is then related to the incubation time to determine enzyme activity.
  • proportions of the polar and less-polar/non-polar solution can be adjusted to ensure proper extraction of each class of analytes and enzyme reconstitution. This will allow new analytes to be added to the test menu with only minor changes to the method.
  • this approach is flexible enough so that if one wants just to measure metabolite markers, one can consolidate the first tow of steps into a single one by making a solution of polar/less polar solvents and in a single step extract both polar and non-polar analytes.
  • a mixture of 75/25 methanol/water (v/v) can extract both polar amino acids and less-polar acylcarnitines in one step and that they can be measured by MS/MS with no prior derivatization.
  • the present invention includes a two-step protocol that does not require sample derivatization and that allows for the simultaneous measurement of metabolite concentrations and enzyme activities and that allows for the simultaneous screening of a multitude of IEMs.
  • the method of the represent invention may also be practiced using the sample test containers and related methods described in co-pending U.S. patent application Ser. No. 09/474,604 by Ostrup, hereby incorporated herein by reference.
  • FIG. 1 is a schematic of a newborn screening method for metabolite concentration measurement by MS/MS in accordance with the prior art. This method is used to extract and quantitate amino acids and acylcarnitines from newborn blood dried on filter paper. The amino acids and acylcarnitines concentration profiles are used to screen fatty acid ⁇ -oxidation, organic acid, and amino acid metabolic disorders in newborns (such as shown in U.S. Pat. Nos. 6,258,605 B1 and 6,455,321 B1 to Chace; hereby incorporated herein by reference).
  • FIG. 2 is a schematic of a newborn screening method for enzyme activity measurement by fluorometry in accordance with the prior art.
  • This method developed by Akie Fujimoto, et. al 7 is designed to screen for galactosemia by reconstituting the enzyme galactose-1-phospate uridyltransferase (GALT) from newborn dried blood spots, adding a fluorescent artificial substrate and monitor the rate of substrate to product conversion by fluorometry.
  • GALT galactose-1-phospate uridyltransferase
  • the enzyme activity information is used to determine whether a newborn may be afflicted with galactosemia.
  • FIG. 3 shows a schematic of an assay procedure in accordance with one embodiment of the invention.
  • FIG. 3 shows that the approaches exemplified in FIGS. 1 and 2 are consolidated in the present invention using the following procedure: Dried blood spots (DBS) may be punched into one or more microtiter well(s).
  • DBS Dried blood spots
  • the enzyme of interest and polar analytes e.g. amino acids
  • a relative polar solution e.g. 100% water.
  • This solution may contain all of the necessary internal standards and substrates.
  • the mixture is then incubated to allow enzyme activity and analyte extraction.
  • a relatively non-polar solvent e.g., 100% MeOH
  • non-polar analytes e.g. acylcarnitines
  • This second solution may contain all of the necessary internal standards. Enzyme precipitation and analyte extraction are allowed to occur. The enzymatic product, polar analytes and non-polar analytes may then be analyzed/quantified by tandem mass spectrometry. The analyte concentration and enzyme activity information is then used to determine whether the newborn is afflicted with any inborn error of metabolism.
  • FIG. 4 shows a schematic of an alternative assay procedure in accordance with another embodiment of the invention.
  • FIG. 4 shows that dried blood spots (DBS) may be punched into one or more microtiter well(s). The wells are already coated will all necessary internal standards and substrates.
  • the enzyme and the polar analytes e.g. amino acids
  • a relative polar solution e.g. 100% water
  • the mixture is then incubated to allow enzyme activity.
  • a relatively non-polar solvent e.g., 100% MeOH
  • a relatively non-polar analytes e.g., 100% MeOH
  • Enzyme precipitation and analyte extraction are allowed to occur.
  • the enzymatic product, polar analytes and non-polar analytes may then be analyzed/quantified by tandem mass spectrometry.
  • the analyte concentration and enzyme activity information is then used to determine whether the newborn is afflicted with any inborn error of metabolism.

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Application Number Priority Date Filing Date Title
US10/652,732 US20050048499A1 (en) 2003-08-29 2003-08-29 Tandem mass spectrometry method for the genetic screening of inborn errors of metabolism in newborns
CA2537034A CA2537034C (en) 2003-08-29 2004-08-30 Mass spectrometry methods for simultaneous detection of metabolic enzyme activity and metabolite levels
EP04782672.2A EP1664325B1 (en) 2003-08-29 2004-08-30 Mass spectrometry methods for simultaneous detection of metabolic enzyme activity and metabolite levels
JP2006524947A JP4838129B2 (ja) 2003-08-29 2004-08-30 代謝酵素活性及び代謝産物レベルの同時検出のための質量分析法
AU2004269410A AU2004269410B2 (en) 2003-08-29 2004-08-30 Mass spectrometry methods for simultaneous detection of metabolic enzyme activity and metabolite levels
ES04782672.2T ES2527306T3 (es) 2003-08-29 2004-08-30 Métodos de espectrometría de masas para la detección simultánea de actividad de enzimas metabólicas y niveles de metabolitos
US10/539,273 US20060234326A1 (en) 2003-08-29 2004-08-30 Mass spectrometry methods for simultaneous detection of metabolic enzyme activity and metabolite levels
PCT/US2004/028238 WO2005021779A1 (en) 2003-08-29 2004-08-30 Mass spectrometry methods for simultaneous detection of metabolic enzyme activity and metabolite levels
US12/349,669 US8318417B2 (en) 2003-08-29 2009-01-07 Simultaneous detection of metabolic enzyme activity and metabolite levels
JP2011126859A JP2011167208A (ja) 2003-08-29 2011-06-07 代謝酵素活性及び代謝産物レベルの同時検出のための質量分析法
US13/357,324 US8399186B2 (en) 2003-08-29 2012-01-24 Simultaneous detection of metabolic enzyme activity and metabolite levels

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US10/539,180 Continuation US7485435B2 (en) 2003-08-29 2005-02-28 Simultaneous detection of metabolic enzyme activity and metabolite levels
US11/539,180 Continuation US7805151B2 (en) 2005-10-06 2006-10-06 System for substantially simultaneous alerts

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US12/349,669 Active 2026-06-25 US8318417B2 (en) 2003-08-29 2009-01-07 Simultaneous detection of metabolic enzyme activity and metabolite levels
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US20060257963A1 (en) * 2004-08-30 2006-11-16 Blas Cerda Simultaneous detection of metabolic enzyme activity and metabolite levels
US20070077548A1 (en) * 2005-05-20 2007-04-05 Gerhild Boger Method for determination of cardiovascular risk factors in dried blood
US20090111137A1 (en) * 2003-08-29 2009-04-30 Perkinelmer Las, Inc. Simultaneous detection of metabolic enzyme activity and metabolite levels
CN102369292A (zh) * 2009-03-16 2012-03-07 华莱克有限公司 生物素酰胺酶测定
CN109416926A (zh) * 2016-04-11 2019-03-01 迪森德克斯公司 质谱数据分析工作流程
CN111272888A (zh) * 2020-01-10 2020-06-12 山东英盛生物技术有限公司 一种新生儿血片中氨基酸及肉碱筛查预处理方法

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