US20150168421A1

US20150168421A1 - Srm methods in alzheimer's disease and neurological disease assays

Info

Publication number: US20150168421A1
Application number: US14/390,447
Authority: US
Inventors: Paul Edward Kearney; Xiao-Jun Li; Clive Hayward
Original assignee: Integrated Diagnostics Inc
Current assignee: Integrated Diagnostics Inc
Priority date: 2012-04-05
Filing date: 2013-03-14
Publication date: 2015-06-18
Also published as: US20180284128A1; US20170299604A1; US11467167B2; WO2013151726A1; US20170299605A1; US20200348310A1

Abstract

Provided herein are methods for developing selected reaction monitoring mass spectrometry (LC-SRM-MS) assays.

Description

RELATED APPLICATIONS

This application claims priority and benefit of U.S. Provisional Application No. 61/620,770, filed Apr. 5, 2012, the contents of which is incorporated by reference in it's entirety.

BACKGROUND

Liquid Chromatography Selected Reaction Monitoring Mass Spectrometry (LC-SRM-MS) has emerged as an alternative technology to immunoassays for quantification of target proteins in biological samples. LC-SRM-MS methods are highly desirable because LC-SRM-MS methods provide both absolute structural specificity for the target protein and relative or absolute measurement of the target protein concentration when suitable internal standards are utilized. In contrast to immunoassays, LC-SRM-MS does not involve the manufacturing of biologics. LC-SRM-MS protein assays can be rapidly and inexpensively developed in contrast to the development of immunoassays. LC-SRM-MS are highly multiplexed, with simultaneous assays for hundreds of proteins performed in a single sample analysis. Using LC-SRM-MS in contrast to other proteomic technologies allows for complex assays for the identification diagnostic proteins in complex diseases such as cancer, autoimmune, and metabolic disease. In particular, the development of a highly multiplexed LC-SRM-MS assay that reproducibly identifies a specific set of proteins relevant to a clinical disease presents diagnostic advantages and efficiencies. To date, proteomic techniques have not enabled such assays to exist where hundreds of proteins can be accurately quantified within a single sample. The present disclosure provides accurate measurement of hundreds of Alzheimer's disease associated proteins within a single sample using multiplexed techniques.

SUMMARY

The present disclosure provides a LC-SRM-MS assay for the measurement of at least 357 Alzheimer's disease associated proteins in a single sample and in a single LC-SRM-MS assay. The assay was optimized for protein quantification and minimal interference among proteins in the assay. This LC-SRM-MS assay is novel because measurement of a large number of proteins in a single sample specifically associated with Alzheimer's disease has not been accomplished. Simultaneous measurement of such a large number of proteins without interference among the proteins requires specific techniques to distinguish among the proteins. The current disclosure provides clinical utility as this assay was used for development of Alzheimer's disease diagnostic tests for the early detection of Alzheimer's disease, managing disease treatment, as well as testing for disease recurrence.
The object of the present disclosure is to provide improved methods for the use of LC-SRM-MS in the development of assays. Accordingly, provided herein is a method for developing peptides and transitions for a plurality of at least 200 proteins for a single sample selected reaction monitoring mass spectrometry (LC-SRM-MS) assay, including the steps of providing a set of 200 or more proteins; generating transitions for each protein; determining the Mascot score for SRM-triggered tandem mass spectrometry (MS/MS) spectra; performing collision energy optimization on the transitions; selecting peptides with transitions showing the greatest peak areas of their transitions; selecting a set of transitions for each peptide, wherein the transitions for each peptide have one of the four most intense b or y transition ions; the transitions for each peptide have m/z values of at least 30 m/z above or below those of the precursor ion; the transitions for each peptide do not interfere with transitions from other peptides; and the transitions represent transitions due to breakage of peptide bond at different sites of the protein.
In one embodiment of the method, each selected peptide in the set of peptides has a monoisotopic mass of 700-5000 Da; and does not contain a cysteine or a methionine or does not contain cysteine or methionine. In other embodiments, each selected peptide contains cysteine or methionine. In another embodiment, the transitions for each peptide have one of the four most intense b or y transition ions; have m/z values of at least 30 m/z above or below those of a precursor ion; do not interfere with transitions from other peptides; and represent transitions due to breakage of peptide bond at different sites of the protein.
In another embodiment of the method, the peptides do not include any peptide that is bounded by KK, KR, RK or RR (either upstream or downstream) in the corresponding protein sequence. Specifically, the amino acid is charged at pH 7.0. In another embodiment, each peptide of said set of peptides is unique to the corresponding protein. In yet another embodiment, the peptides do not include peptides which were observed in post-translational modified forms. In still another embodiment, each set of peptides is prioritized according to one or more of the following ordered set of criteria: unique peptides first, then non-unique; peptides with no observed post-translational modifications first, then those observed with post-translational modifications; peptides within the mass range 800-3500 Da first, then those outside of 800-3500 Da; and sorted by decreasing number of variant residues. In certain embodiments, the peptides are unique in that they only appear once among the peptides run in a single assay.
In one embodiment, each set of peptides is prioritized according to all of the ordered set of criteria. In another embodiment, each prioritized set of peptides contains 1-5 peptides.
In certain embodiments of the preceding methods, the two best peptides per protein and the two best transitions per peptide are selected based on experimental data resulting from LC-SRM-MS analysis of one or more of the following experimental samples: a biological disease sample, a biological control sample, and a mixture of synthetic peptides of interest. In a particular embodiment, the biological disease and biological control samples are processed using an immunodepletion method prior to LC-SRM-MS analysis. In another embodiment, the experimental samples contain internal standard peptides. In yet another embodiment, the LC-SRM-MS analysis method specifies a maximum of 7000 transitions, including transitions of the internal standard peptides and transitions. In other embodiments the method specifies a maximum of between 1000-7000, 2000-6000, 3000-5000 and about 3500 transitions.
In one embodiment of the method, the top two transitions per peptide are selected according to one or more of the following criteria the transitions exhibit the largest peak areas measured in either of the two biological experimental samples; the transitions are not interfered with by other ions; the transitions do not exhibit an elution profile that visually differs from those of other transitions of the same peptide; or the transitions are not beyond the detection limit of both of the two biological experimental samples.
In another embodiment of the method, the top two peptides per protein are selected according to one or more of the following criteria: one or more peptides exhibit two transitions and represent the largest combined peak areas of the two transitions; or one or more peptides exhibit one transition and represent the largest combined peak areas of the two transitions.
In another aspect, provided herein is an assay developed according to the foregoing method, and embodiments thereof.
In yet another aspect provided herein is the use of an assay developed according to the foregoing method, and embodiments thereof, to detect a plurality of at least 200 proteins in a single biological sample.
In another aspect, provided herein is an assay developed according to the foregoing method, and embodiments thereof.
The disclosure provides a use of a composition, as described above, for the development of an assay to detect a disease, disorder or condition in a mammal.
The disclosure provides a method comprising analyzing a composition, as described above, using mass spectrometry. The method can use selected reaction monitoring mass spectrometry.

DETAILED DESCRIPTION

The present disclosure relates to methods for developing peptides and transitions for a single sample selected reaction monitoring mass spectrometry (LC-SRM-MS) assay, generally comprising the steps of providing a set of proteins; identifying representative proteolytic peptides for each protein according to a set of criteria; identifying representative transitions for each peptide according to another set of criteria; and selecting the optimum peptides per protein and the optimum transitions per peptide.
Selected reaction monitoring mass spectrometry is capable of highly sensitive and accurate protein quantification based on the quantification of proteolytic peptides. In terms of clinical utility, mass spectrometry-based assays are often compared to immunoassays (e.g., Enzyme-Linked Immunosorbent Assay, or ELISA), which have the ability to quantify specific analytes in large sample sets (e.g., 96 or 384 samples in parallel microtitre plate-based format). Until recently, mass spectrometry-based protein assays were not able to match these sample sizes or quantitative accuracy. Considerable time and expense is required to generate and characterize antibodies required for immunoassays. Increasingly efficient LC-SRM-MS assays, therefore, may surpass immunoassays such as ELISA in the rapid development of clinically useful, multiplexed protein assays.
LC-SRM-MS is a highly selective method of tandem mass spectrometry which has the potential to effectively filter out all molecules and contaminants except the desired analyte(s). This is particularly beneficial if the analysis sample is a complex mixture which may comprise several isobaric species within a defined analytical window. LC-SRM-MS methods may utilize a triple quadrupole mass spectrometer which, as is known in the art, includes three quadrupole rod sets. A first stage of mass selection is performed in the first quadrupole rod set, and the selectively transmitted ions are fragmented in the second quadrupole rod set. The resultant transition (product) ions are conveyed to the third quadrupole rod set, which performs a second stage of mass selection. The product ions transmitted through the third quadrupole rod set are measured by a detector, which generates a signal representative of the numbers of selectively transmitted product ions. The RF and DC potentials applied to the first and third quadrupoles are tuned to select (respectively) precursor and product ions that have m/z values lying within narrow specified ranges. By specifying the appropriate transitions (m/z values of precursor and product ions), a peptide corresponding to a targeted protein may be measured with high degrees of sensitivity and selectivity. Signal-to-noise ratio in LC_SRM_MS is often superior to conventional tandem mass spectrometry (MS/MS) experiments, that do not selectively target (filter) particular analytes but rather aim to survey all analytes in the sample.
Accordingly, provided herein is a method for developing peptides and transitions for a plurality of proteins for use in selected reaction monitoring mass spectrometry (LC-SRM-MS) assay. In a preferred embodiment, the assay involves the analysis of a single sample containing all analytes of interest (e.g., a proteolytic digest of plasma proteins). As to the selection of the protease(s) used, trypsin, which cleaves exclusively C-terminal to arginine and lysine residues, is a preferred choice to generate peptides because the masses of generated peptides are compatible with the detection ability of most mass spectrometers (up to 2000 m/z), the number and average length of generated peptides, and also the availability of efficient algorithms for the generation of databases of theoretical trypsin-generated peptides. High cleavage specificity, availability, and cost are other advantages of trypsin. Other suitable proteases will be known to those of skill in the art. Miscleavage is a factor for failure or ambiguous protein identification. A miscleavage can be defined as partial enzymatic protein cleavages generating peptides with internal missed cleavage sites reflecting the allowed number of sites (targeted amino acids) per peptide that were not cut. The presence of post-translational modifications (PTMs) is also a potential contributor to the problem of miscleavages.
LC-SRM-MS mass spectrometry involves the fragmentation of gas phase ions and occurs between the different stages of mass analysis. There are many methods used to fragment the ions and these can result in different types of fragmentation and thus different information about the structure and composition of the molecule. The transition ions observed in an LC-SRM-MS spectrum result from several different factors, which include, but are not limited to, the primary sequence, the amount of internal energy, the means of introducing the energy, and charge state. Transitions must carry at least one charge to be detected. An ion is categorized as either a, b or c if the charge is on a transition comprising the original N terminus of the peptide, whereas the ion is categorized as either x, y or z if the charge is on a transition comprising the original C terminus of the peptide. A subscript indicates the number of residues in the transition (e.g., one peptide residue in x₁, two peptide residues in y₂, and three peptide residues in z₃, etc.).
In a generic peptide repeat unit represented —N—C(O)—C—, an x ion and an a ion resulting from cleavage of the carbonyl-carbon bond (i.e., C(O)—C). The x ion is an acylium ion, and the a ion is an iminium ion. A y ion and a b ion result from cleavage of the carbonyl-nitrogen bond (i.e., C(O)—N, also known as the amide bond). In this case, the y ion is an ammonium ion and the b ion is an acylium ion. Finally, a z ion and a c ion result from cleavage of the nitrogen-carbon (i.e., C—N) bond. The z ion is a carbocation and the c ion is an ammonium ion.
Superscripts are sometimes used to indicate neutral losses in addition to the backbone fragmentation, for example, * for loss of ammonia and ° for loss of water. In addition to protons, c ions and y ions may abstract an additional proton from the precursor peptide. In electrospray ionization, tryptic peptides may carry more than one charge.
Internal transitions arise from double backbone cleavage. These may be formed by a combination of b-type and y-type cleavage (i.e., cleavage producing b and y ions). Internal cleavage ions may also be formed by a combination of a-type and y-type cleavage. An internal transition with a single side chain formed by a combination of a-type and y-type cleavage is called an iminium ion (sometimes also referred to as an imonium or immonium ion). These ions are labeled with the one letter code for the corresponding amino acid.
Low energy CID (i.e., collision induced dissociation in a triple quadrupole or an ion trap) involves the fragmentation of a peptide carrying a positive charge, primarily along its backbone, to generate primarily a, b and y ions.
In one aspect, provided herein is a method for developing peptides and transitions for a plurality of proteins for a single sample selected reaction monitoring mass spectrometry (LC-SRM-MS) assay: (a) providing a panel or plurality of proteins; (b) identifying a set of peptides for each protein, wherein (i) each peptide in the set of peptides corresponds to a transition of said protein; (ii) the peptides have a monoisotopic mass of 700-5000 Da; and (iii) the peptides do not contain cysteine or does not contain cysteine or methionine. In other embodiments, each selected peptide contains cysteine or methionine. ; and; (c) identifying a set of transitions for each peptide, wherein (i) the transitions for each peptide have one of the four most intense b or y transition ions; (ii) the transitions for each peptide have m/z values of at least 30 m/z above or below those of the precursor ion; (iii) the transitions for each peptide do not interfere with transitions from other peptides; and (iv) the transitions represent transitions due to breakage of peptide bond at different sites of the protein; and (d) selecting the peptides for each protein that best fit the criteria of step (b) and the transitions per peptide that best fit the criteria of step (c); thereby developing peptides and transitions for a LC-SRM-MS assay.
By plurality of proteins it is meant that at least 2, 3, 4, 5, 6, 7, 8, 9, 10, 15, 20, 25, 50, 100, 150, 200, 250, 300, 400, 450, 500 or more proteins. In certain embodiments, the plurality of proteins can encompass between 2 and 10, 10 and 20, 20 and 50, 50 and 100, 100 and 200 or 200 and 500 proteins. In other embodiments, the plurality of proteins can encompass between 250 and 450; or 300 and 400 proteins.
Trypsin-like proteases cleave peptide bonds following a positively charged amino acid (e.g., lysine (K) or arginine (R)). This specificity is driven by the residue which lies at the base of the enzyme's S1 pocket (generally a negatively charged aspartic acid or glutamic acid). Accordingly, in one embodiment of the method, the peptides do not include any peptide that is bounded by KK, KR, RK or RR, either upstream of downstream in the corresponding protein sequence. In another embodiment, each peptide of said set of peptides is unique to the corresponding protein.
Post-translational modification (PTM) is the chemical modification of a protein after its translation. It can include any modification following translation, including cleavage. It is one of the later steps in protein biosynthesis, and thus gene expression, for many proteins. It is desirable to avoid such peptides for the purpose of protein identification. Thus, in another embodiment, the peptides do not include peptides which were observed in post-translational modified forms.
In still another embodiment, each set of peptides is prioritized according to one or more of the following ordered set of criteria: (a) unique peptides first, then non-unique; (b) peptides with no observed post-translational modifications first, then those observed with post-translational modifications; (c) peptides within the mass range 800-3500 Da first, then those outside of 800-3500 Da; and (d) sorted by decreasing number of variant residues. In one embodiment, each set of peptides is prioritized according to all of the ordered set of criteria. In another embodiment, each prioritized set of peptides contains 1-5 peptides.
In certain embodiments, one or more liquid chromatography (LC) purification steps are performed prior to a subsequent LC-SRM-MS analysis step. Traditional LC analysis relies on the chemical interactions between sample components and column packing materials, where laminar flow of the sample through the column is the basis for separation of the analyte of interest from the test sample. The skilled artisan will understand that separation in such columns is a diffusional process. A variety of column packing materials are available for chromatographic separation of samples, and selection of an appropriate separation protocol is an empirical process that depends on the sample characteristics, the analyte of interest, the interfering substances present and their characteristics, etc. Various packing chemistries can be used depending on the needs (e.g., structure, polarity, and solubility of compounds being purified). In various embodiments the columns are polar, ion exchange (both cation and anion), hydrophobic interaction, phenyl, C-2, C-8, C-18 columns, polar coating on porous polymer, or others that are commercially available. During chromatography, the separation of materials is effected by variables such as choice of eluant (also known as a “mobile phase”), choice of gradient elution and the gradient conditions, temperature, etc. In certain embodiments, an analyte may be purified by applying a sample to a column under conditions where the analyte of interest is reversibly retained by the column packing material, while one or more other materials are not retained. In these embodiments, a first mobile phase condition can be employed where the analyte of interest is retained by the column, and a second mobile phase condition can subsequently be employed to remove retained material from the column, once the non-retained materials are washed through. Alternatively, an analyte may be purified by applying a sample to a column under mobile phase conditions where the analyte of interest elutes at a differential rate in comparison to one or more other materials. As discussed above, such procedures may enrich the amount of one or more analytes of interest relative to one or more other components of the sample.
The following parameters are used to specify an LC-SRM-MS assay of a protein under a particular LC-SRM-MS system: (1) a tryptic peptide of the protein; (2) the retention time (RT) of the peptide; (3) the m/z value of the peptide precursor ion; (4) the declustering potential used to ionize the precursor ion; (5) m/z value of a fragment ion generated from the peptide precursor ion; and (6) the collision energy (CE) used to fragment the peptide precursor ion that is optimized for the particular peptide.
In certain embodiments of the preceding methods, the two best peptides per protein and the two best transitions per peptide are selected based on experimental data resulting from LC-SRM-MS analysis of one or more of the following experimental samples: a biological disease sample, a biological control sample, and a mixture of synthetic peptides of interest. Biological samples include body fluids, tissue samples and cell samples. Body fluid samples can include blood, serum, sputum, genital secretions, cerebrospinal fluid, sweat or excreta such as urine. Body tissue samples can include lung, skin, brain, spine, bone, muscle, epithelial, liver, kidney, pancreas, gastrointestinal tract, cardiovascular tissue, heart or nervous tissue. Biological disease samples can include cancer, benign tumors, infected tissue and tissue subject to trauma. In a particular embodiment, the biological disease and biological control samples are processed using an immunodepletion method prior to LC-SRM-MS analysis. Immunodepletion involves removal of one or more proteins through the use of antibodies. Numerous immunodepletion techniques are known to those of skill in the art. In another embodiment, the biological disease and biological control samples are processed using an immunocapture method prior to LC-SRM-MS analysis. Immunocapture involves selection of one or more proteins through the use of antibodies. Numerous immunocapture techniques are known to those of skill in the art.
To facilitate accurate quantification of the peptide transitions by the methods disclosed herein, a set of isotopically-labeled synthetic versions of the peptides of interest may be added in known amounts to the sample for use as internal standards. Since the isotopically-labeled peptides have physical and chemical properties identical to the corresponding surrogate peptide, they co-elute from the chromatographic column and are easily identifiable on the resultant mass spectrum. The addition of the labeled standards may occur before or after proteolytic digestion. Methods of synthesizing isotopically-labeled peptides will be known to those of skill in the art. Thus, in another embodiment, the experimental samples contain internal standard peptides. Other embodiments may utilize external standards or other expedients for peptide quantification.
In yet another embodiment, the LC-SRM-MS analysis method specifies a maximum of 7000 transitions, including transitions of the internal standard peptides and transitions. As used herein, the term “transition” refers to the specific pair of m/z (mass-to-charge) values associated with the precursor and transition ions corresponding to a specific peptide and, therefore, to a specific protein.
In one embodiment of the method, the top two transitions per peptide are selected according to one or more of the following criteria (A): (1) the transitions exhibit the largest peak areas measured in either of the two biological experimental samples; (2) the transitions are not interfered with by other ions; (3) the transitions do not exhibit an elution profile that visually differs from those of other transitions of the same peptide; (4) the transitions are not beyond the detection limit of both of the two biological experimental samples; (5) the transitions do not exhibit interferences.
For the mass spectrometric analysis of a particular peptide, the quantities of the peptide transitions in the sample may be determined by integration of the relevant mass spectral peak areas, as known in the prior art. When isotopically-labeled internal standards are used, as described above, the quantities of the peptide transitions of interest are established via an empirically-derived or predicted relationship between peptide transition quantity (which may be expressed as concentration) and the area ratio of the peptide transition and internal standard peaks at specified transitions.
In another embodiment of the method, the top two peptides per protein are selected according to one or more of the following criteria (B): (1) one or more peptides exhibit two transitions according to criteria (A) and represent the largest combined peak areas of the two transitions according to criteria (A); and (2) one or more peptides exhibit one transition according to criteria (A) and represent the largest combined peak areas of the two transitions according to criteria (A).

Assays

The methods of the present disclosure allow the quantification of high abundance and low abundance plasma proteins that serve as detectable markers for various health states (including diseases and disorders), thus forming the basis for assays that can be used to determine the differences between normal levels of detectable markers and changes of such detectable markers that are indicative of changes in health status. In one aspect of the disclosure, provided herein is an assay developed according to the foregoing method, and embodiments thereof. In another aspect, provided herein is the use of an assay developed according to the foregoing method, and embodiments thereof, to detect a plurality of at least 200, 300 or more proteins in a single sample.

Definitions

As used herein, “transition” refers to a pair of m/z values associated with a peptide. Normally, labeled synthetic peptides are used as quality controls in SRM assays. However, for very large SRM assays, labeled peptides are not feasible. However, correlation techniques (Keary, Butler et al. 2008) were used to confirm the identity of protein transitions with high confidence. The correlation between a pair of transitions is obtained from their expression profile over all samples in the training set study detailed below. As expected, transitions from the same peptide are highly correlated. Similarly, transitions from different peptide fragments of the same protein are also highly correlated. In contrast, transitions form different proteins are not highly correlated. This methodology enables a statistical analysis of the quality of the protein's SRM assay. For example, if the correlation of the transitions from the two peptides from the same protein is above 0.5 then there is less than a 5% probability that the assay is false
As used herein, a “tryptic peptide” refers to the peptide that is formed by the treatment of a protein with trypsin.
As used herein, “RT” refers to “retention time”, the elapsed time between injection and elution of an analyte.
As used herein, “m/z” indicates the mass-to-charge ratio of an ion.
As used herein “DP” refers to the “declustering potential”, a voltage potential to dissolvate and dissociate ion clusters. It is also known as “fragmentor voltage” or “ion transfer capillary offset voltage” depending upon the manufacturer.
As used herein, “CE” refers to “collision energy”, the amount of energy precursor ions receive as they are accelerated into the collision cell.
As used herein, “LC-SRM-MS” is an acronym for “selected reaction monitoring” and may be used interchangeably with “LC-MRM-MS”.
As used herein, “MS/MS” represents tandem mass spectrometry, which is a type of mass spectrometry involving multiple stages of mass analysis with some form of fragmentation occurring in between the stages.
As used herein, “ISP” refers to “internal standard peptides”.
As used herein, “HGS” refers to “human gold standard”, which is comprised of a pool of plasma from healthy individuals.
As used herein, “MGF” refers to “Mascot generic file”. Mascot is a search engine that uses mass spectrometry data to identify proteins from primary sequence databases. A Mascot generic file is a plain text (ASCII) file containing peak list information and, optionally, search parameters.
Mascot is a tool for assessing mass spectrometry data against protein sequences. This data can be acquired from any mass spectrometry technique including MALDI-TOF and electrospray ionization MS (including LC-SRM-MS) data. Mascot uses a ‘probability-based MOWSE’ algorithm to estimate the significance of a match (i.e., that the observed transitions correspond to a particular protein). The total score is the absolute probability that the observed match is a random event. They are reported as −10×LOG10(P), where P is the absolute probability. Lower probabilities, therefore, are reported as higher scores. For example, if the absolute probability that an observed match is random is 1×10⁻¹², Mascot reports it as 120.
The disclosure also provides compositions. These compositions can include any of the transition ions described in Table II. These transition ions exist while peptides derived from the proteins in Table II are undergoing analysis with LC-SRM-MS. In one embodiment, the composition includes any of the transition ions described in Table II. In another embodiment, the composition includes any two transition ions described in Table II. In other embodiments, the composition includes, any 3, 4, 5, 6, 7, 8, 9, 10, 11, 12, 13, 14, 15, 16, 17, 18, 19, 20, 25, 30, 35, 40, 45, 50, 55, 60, 65, 70, 75, 80, 85, 90, 95, 100, 110, 120, 130, 140, 150, 160, 170, 180, 190, 200, 210, 220, 230, 240, 250, 260, 270, 280, 290, 300 or 331 transition ions described in Table II.
In another embodiment, each of the transition ions in the composition corresponds and/or is derived from a different protein. In another embodiment, 90% of the transition ions in the composition correspond with and/or are derived from a protein that no other transition ion in the composition corresponds. In other embodiments, 80, 70, 60, 50, 40, 30, 20, 10 or 0% of the transition ions in the composition correspond and/or are derived from a protein that no other transition ion in the composition corresponds.
The compositions described herein included synthetic peptides. Synthetic peptides can be used as controls for the abundance of proteins they are derived from and/or correspond. In certain embodiments, the abundance of the synthetic peptides is defined and the results are compared to LC-SRM-MS results from a peptide found in a sample to the LC-SRM-MS results in the corresponding synthetic peptide. This allows for the calculation of the abundance of the peptide in the sample. In certain embodiments, by knowing the abundance of a peptide in a sample, the abundance of the protein it corresponded to is determined.
Synthetic peptides can be generated using any method known in the art. These methods can include recombinant expression techniques such as expression in bacteria or in vitro expression in eukaryotic cell lysate. These methods can also include solid phase synthesis.
In one embodiment, the composition includes synthetic peptides selected from any of the peptides described in Table II. In another embodiment, the composition included any two peptides described in Table II. In other embodiments, the composition included, any 3, 4, 5, 6, 7, 8, 9, 10, 11, 12, 13, 14, 15, 16, 17, 18, 19, 20, 25, 30, 35, 40, 45, 50, 55, 60, 65, 70, 75, 80, 85, 90, 95, 100, 110, 120, 130, 140, 150, 160, 170, 180, 190, 200, 210, 220, 230, 240, 250, 260, 270, 280, 290, 300, 331 or more peptides described in Table II.
In another embodiment, each of the peptides in the composition each corresponds with a different protein. In another embodiment, 90% of the peptides in the composition correspond with a protein that no other peptide in the composition corresponds with. In other embodiments, 80, 70, 60, 50, 40, 30, 20, 10 or 0% of the peptides in the composition correspond with from a protein that no other peptide in the composition corresponds with.
The peptides can be isotopically labeled. The isotopes with which they can be labeled include ¹³C, ²H, ¹⁵N and ¹⁸O. The peptides can also include a polar solvent. Polar solvents can include water and mixtures of ethanol and water.
In certain embodiments, the samples described herein are taken from mammals. These mammals include rats, mice, rabbits, dogs, non-human primates and humans. Samples can be isolated from any tissue or organ or from any bodily fluid. Organs from which samples can be taken include skin, heart, lung, brain, kidney, liver, pancreas, spleen, testes, ovaries, gall bladder, thymus, thyroid, eye, ear, nose, mouth, tongue, penis, vagina, bladder or larynx. Tissues include nervous tissue, vascular tissue, muscle, bone, gastrointestinal tract, epithelial tissue, fibroblastic tissue, mucous membranes, hair, skin, reproductive tissue and connective tissue. Body fluids and excretions include, blood, serum, saliva, urine, semen, vaginal secretions, excrement, bile, tears, lymph, ear wax, mucous, shed skin, finger nails, toe nails, skin oils, sweat and dandruff.
The relative abundance of one or more of the proteins represented by the transition ions and synthetic peptides described above can be used to diagnose, determine likelihood of the presence of, develop prognoses for and/or stage various diseases and pathologies. Often the organ, tissue or bodily fluid or excretion from which the sample is taken is distinct from the organ, tissue or bodily fluid or excretion involved with the disease or pathology. For example, the presence of Alzheimer's disease can be determined from a sample taken from blood. Any type of body fluid may be used in the assays.
Diseases and pathologies that status, diagnosis, presence or prognosis can be found using the transition ions and/or synthetic peptides described herein include cancer, metabolic diseases, neurological disorders, infectious diseases and cardiovascular disorders.

EXAMPLES

I. Exemplary Standard Operating Procedure

Protein Selection

Proteins known to be over-expressed or under-expressed in Alzheimer's disease patients were obtained (through literature searching, experimental data or proprietary databases) as shown in Table I. The set of proteins was reduced to a set of 357 proteins (see Table II) by prioritizing those proteins that have been previously detected my LC-MS/MS in blood (serum or plasma).
Selected proteins were then identified by their UniProt protein name and accession, their Entrez gene symbol and gene name, the isoform accession and their amino acid sequence. The canonical isoform in UniProt was selected if a protein has more than one isoform.

Peptide Selection for Synthesis

The five best peptides per protein for LC-SRM-MS assay were selected for as follows. Fully tryptic peptides having a monoisotopic mass of 800-3500 mass units, without miscleavages, not containing a cysteine (C) or a methionine (M), without having high miscleavage probability were selected. Further, any peptide that was bounded by KK, KR, RK or RR (either upstream or downstream) in the corresponding protein sequence was not selected.
Peptides were selected that were unique to the protein of interest. Peptides were only selected that match only one protein or protein family including analogues of the one protein, when searched in protein databases. Further, peptides which were observed in post-translational modified forms were not selected. Databases were assessed that showed expression of the proteins from which the peptides were isolated in human blood. Also databases of good quality MS peptides were searched. Peptides that appeared in human blood and were good quality MS peptides were favored. If these methods did not result in a sufficient number of peptides, rules were relaxed in a step wise manner to allow a greater number of peptides until a sufficient number was reached. The purity of the synthesized peptides was >75% and the amount of material was ≧25 μg. Peptides did not need to be desalted.
The four best transitions per peptide are then selected and optimized based on experimental results from a mixture of synthetic peptides. LC-SRM-MS-triggered MS/MS spectra was acquired for each synthetic peptide, using a QTRAP 5500 instrument. One spectrum or the doubly—and one for the triply—charged precursor ion was collected for each of the identified peptides (Mascot score ≧15), retention time was recorded for the four most intense b or y transition ions. The selected transition ions possessed m/z values were at least 30 m/z above or below those of the precursor ions; they did not interfere with other synthetic peptides; and they were transition ions due to breakage of peptide bond at different sites.
If an insufficient percentage of the synthetic peptides were acquired, the steps were repeated. In some cases, the second transition with first with theoretical y+ ions with m/z values at least 30 m/z above those of the doubly charged precursor ion was selected if an insufficient percentage was acquired. Peptides that failed to trigger the acquisition of MS/MS spectrum were discarded.

II. Exemplary Protein list

The abundance of the following proteins can be assessed substantially simultaneously using the MS-LC-SRM-MS system described herein. Transitions from these proteins can be used to diagnose diseases including Alzheimer's disease when their abundance is measured in a biological specimen from a subject to be diagnosed for Alzheimer's disease. In one embodiment, the abundances of these proteins are measure in the blood serum of the subject.

Lengthy table referenced here
US20150168421A1-20150618-T00001
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Lengthy table referenced here
US20150168421A1-20150618-T00002
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VI. Exemplary Assayed Protein

The expression of the following 357 proteins were assessed substantially simultaneously using the MS-LC-SRM-MS system described herein.
41_HUMAN
5HT2C_HUMAN
A1AG1_HUMAN
A1AG2_HUMAN
A1BG_HUMAN
A2MG_HUMAN
A4_HUMAN
AACT_HUMAN
ABCA1_HUMAN
ACBD7_HUMAN
ACE2_HUMAN
ACHA2_HUMAN
ACHA4_HUMAN
ACHAS_HUMAN
ACHB_HUMAN
ACHB2_HUMAN
ADA12_HUMAN
ADA23_HUMAN
AFAM_HUMAN
AGAL_HUMAN
AGAP2_HUMAN
ALBU_HUMAN
ALS_HUMAN
AMFR2_HUMAN
AMNLS_HUMAN
AMPB_HUMAN
ANGP1_HUMAN
ANGT_HUMAN
ANO3_HUMAN
ANT3_HUMAN
AP1B1_HUMAN
APC2_HUMAN
APLP1_HUMAN
APOA1_HUMAN
AP0A2_HUMAN
AP0A4_HUMAN
APOB_HUMAN
APOC2_HUMAN
APOD_HUMAN
APOE_HUMAN
APOL4_HUMAN
APOOL_HUMAN
ARHG7_HUMAN
ARP21_HUMAN
ARSA_HUMAN
ARSE_HUMAN
ARTN_HUMAN
ASGR1_HUMAN
AT12A_HUMAN
AT2A2_HUMAN
AT2B3_HUMAN
ATS1_HUMAN
BAX_HUMAN
BCAS1_HUMAN
BDNF_HUMAN
BEST1_HUMAN
BTNL8_HUMAN
C1QL2_HUMAN
C1QT4_HUMAN
CACB2_HUMAN
CAD11_HUMAN
CAD19_HUMAN
CAD22_HUMAN
CADH3_HUMAN
CADH5_HUMAN
CADH7_HUMAN
CALL3_HUMAN
CAMKV_HUMAN
CAR14_HUMAN
CATD_HUMAN
CB080_HUMAN
CB085_HUMAN
CBPN_HUMAN
CD3D_HUMAN
CD72_HUMAN
CEL3A_HUMAN
CEL3B_HUMAN
CERU_HUMAN
CETP_HUMAN
CF072_HUMAN
CFAB_HUMAN
CFAH_HUMAN
CHAD_HUMAN
CK041_HUMAN
CLC4M_HUMAN
CLUS_HUMAN
CNTN1_HUMAN
CNTN2_HUMAN
CO1A2_HUMAN
CO2_HUMAN
CO3_HUMAN
CO4A_HUMAN
CO4A4_HUMAN
CO4B_HUMAN
C06_HUMAN
CO8A_HUMAN
CO9A2_HUMAN
COIA1_HUMAN
CORT_HUMAN
CP46A_HUMAN
CPLX2_HUMAN
CRLF1_HUMAN
CRUM1_HUMAN
CSF1_HUMAN
CSF1R_HUMAN
DBC1_HUMAN
DCBD1_HUMAN
DCBD2_HUMAN
DDR2_HUMAN
DIRA2_HUMAN
E41L3_HUMAN
EAA2_HUMAN
EDNRB_HUMAN
ELAV3_HUMAN
EMIL2_HUMAN
EMIL3_HUMAN
EPHA8_HUMAN
ERLN1_HUMAN
ERMIN_HUMAN
ERO1B_HUMAN
F123A_HUMAN
F13A_HUMAN
FA20A_HUMAN
FCGRN_HUMAN
FETUA_HUMAN
FEZ1_HUMAN
FGFR2_HUMAN
FGFR3_HUMAN
FGL1_HUMAN
FIBA_HUMAN
FIBB _HUMAN
FIBG_HUMAN
FINC_HUMAN
FRS2_HUMAN
GABR2_HUMAN
GALR3_HUMAN
GAS6_HUMAN
GBRA2_HUMAN
GBRB2_HUMAN
GELS_HUMAN
GFRA2_HUMAN
GNAQ_HUMAN
GOLM1_HUMAN
GOPC_HUMAN
GP113_HUMAN
GP125_HUMAN
GP158_HUMAN
GP2_HUMAN
GPC5_HUMAN
GPC5D_HUMAN
GPC6_HUMAN
GPR88_HUMAN
GRIA2_HUMAN
GRM5_HUMAN
GRN_HUMAN
GT253_HUMAN
HAS1_HUMAN
HCN1_HUMAN
HCN2_HUMAN
HEMO_HUMAN
HEP2_HUMAN
HPCA_HUMAN
HPT_HUMAN
HRG_HUMAN
HS3S5_HUMAN
I12R1_HUMAN
IC1_HUMAN
ICAM3_HUMAN
IGF1R_HUMAN
IL12B _HUMAN
IL1AP_HUMAN
IL1R2_HUMAN
INADL_HUMAN
INHBA_HUMAN
IPSP_HUMAN
ITA3_HUMAN
ITAM_HUMAN
ITB2_HUMAN
ITB5_HUMAN
ITIH1_HUMAN
ITIH2_HUMAN
ITIH3_HUMAN
ITIH4_HUMAN
JPH3_HUMAN
KAIN_HUMAN
KALRN_HUMAN
KCC1G_HUMAN
KCC2A_HUMAN
KCNA1_HUMAN
KCNA2_HUMAN
KCNA3_HUMAN
KCNA5_HUMAN
KCNQ1_HUMAN
KCNV2_HUMAN
KCTD4_HUMAN
KIF5A_HUMAN
KIRR2_HUMAN
KLK3_HUMAN
KLKB1_HUMAN
KNG1_HUMAN
KSYK_HUMAN
LAMB2_HUMAN
LAT2_HUMAN
LAT3_HUMAN
LCK_HUMAN
LCN8_HUMAN
LGI1_HUMAN
LGMN_HUMAN
LIPE_HUMAN
LRMP_HUMAN
LRP8_HUMAN
LRTM2_HUMAN
LSHR_HUMAN
LTBP1_HUMAN
LYG2_HUMAN
MAMC2_HUMAN
MAP4_HUMAN
MICA_HUMAN
MMP1_HUMAN
MMP16_HUMAN
MMP17_HUMAN
MMP2_OHUMAN
MMP24_HUMAN
MMP9_HUMAN
MOT2_HUMAN
MPDZ_HUMAN
MTOR_HUMAN
MYP2_HUMAN
NCAN_HUMAN
NCIOC2_HUMAN
NDF6_HUMAN
NECP2_HUMAN
NETO1_HUMAN
NETR_HUMAN
NEUG_HUMAN
NEUM_HUMAN
NFL_HUMAN
NKX62_HUMAN
NMDE1_HUMAN
NMDE3_HUMAN
NMDZ1_HUMAN
NMS_HUMAN
NOE3_HUMAN
NPT4_HUMAN
NPTX1_HUMAN
NRG3_HUMAN
NTRK2_HUMAN
ODP2_HUMAN
OLFL3_HUMAN
OLIG1_HUMAN
OPCM_HUMAN
OTOAN_HUMAN
P2RX1_HUMAN
P4K2A_HUMAN
PACN1_HUMAN
PAK3_HUMAN
PAQR6_HUMAN
PAR6B_HUMAN
PARD3_HUMAN
PARK7_HUMAN
PCD1S_HUMAN
PCDA5_HUMAN
PCDAA_HUMAN
PCDB6_HUMAN
PCDB7_HUMAN
PCDBC_HUMAN
PCDBF_HUMAN
PCDGE_HUMAN
PCDGF_HUMAN
PCSK1_HUMAN
PDIA2_HUMAN
PDYN_HUMAN
PEDF_HUMAN
PERL_HUMAN
PGCB_HUMAN
PGCP_HUMAN
PICAL_HUMAN
PIN1_HUMAN
PKDRE_HUMAN
PLCB1_HUMAN
PON1_HUMAN
PRIO_HUMAN
PSMG1_HUMAN
PTN5_HUMAN
PTPRB_HUMAN
PTPRO_HUMAN
PTPRT_HUMAN
PVRL1_HUMAN
PZP_HUMAN
RCN1_HUMAN
RELN_HUMAN
RES18_HUMAN
RGS11_HUMAN
RGS2O_HUMAN
RGS4_HUMAN
RRAGC_HUMAN
RUN3A_HUMAN
S12A5_HUMAN
S12A6_HUMAN
S15A2_HUMAN
S39A4_HUMAN
SAA4_HUMAN
SCG1_HUMAN
SCG3_HUMAN
SCN2A_HUMAN
SCNNA_HUMAN
SCRT1_HUMAN
SEM4A_HUMAN
SEMG1_HUMAN
SEPP1_HUMAN
SEPT3_HUMAN
SGCZ_HUMAN
SHSA7_HUMAN
SIA8C_HUMAN
SIG12_HUMAN
SIX3_HUMAN
SLIK1_HUMAN
SLIT1_HUMAN
SNP25_HUMAN
SNTB1_HUMAN
SO1A2_HUMAN
SO1B3_HUMAN
SPB5_HUMAN
SREC_HUMAN
STH_HUMAN
SYN2_HUMAN
SYNPR_HUMAN
SYTL4_HUMAN
SYUA_HUMAN
SYUB_HUMAN
T151A_HUMAN
TADBP_HUMAN
TAU_HUMAN
TBB2B_HUMAN
TERA_HUMAN
TFR2_HUMAN
TLR7_HUMAN
TM9S1_HUMAN
TMPS2_HUMAN
TNF6B _HUMAN
TNR19_HUMAN
TR11B _HUMAN
TRFR_HUMAN
TRIM9_HUMAN
TRPV5_HUMAN
TYRO_HUMAN
UGGG2_HUMAN
UNC5C_HUMAN
VGFR3_HUMAN
VTDB_HUMAN
VTNC_HUMAN
WNK4_HUMAN
WNT8B _HUMAN
XLRS1_HUMAN
YQ051_HUMAN
ZIC1_HUMAN
ZIC2_HUMAN

LENGTHY TABLES
The patent application contains a lengthy table section. A copy of the table is available in electronic form from the USPTO web site (http://seqdata.uspto.gov/?pageRequest=docDetail&DocID=US20150168421A1). An electronic copy of the table will also be available from the USPTO upon request and payment of the fee set forth in 37 CFR 1.19(b)(3).

Claims

1. A multiplexed LC-SRM-MS assay for the measurement of a plurality of proteins in a single sample comprising:

a) generating a set of optimal peptides and corresponding transitions for each protein monitored;

b) optimizing the collision energy for each transition such that interference among the transitions monitored is avoided;

c) selecting a set of transitions that have the greatest peak areas are monitored for each of the proteins, and wherein the selected transitions do not interfere with the ions in the sample;

d) monitoring the detected set of transitions for each protein in the sample, there-by measuring a plurality of proteins in the sample.

2. The assay of claim 1, wherein each monitored peptide

(i) has a monoisotopic mass of 700-5000 Da; and

(ii) does not contain a cysteine or a methionine; and.

3. The assay of claim 1, wherein the transitions for each peptide

(i) have one of the four most intense b or y transition ions;

(ii) has m/z values of at least 30 m/z above or below those of a precursor ion;

(iii) do not interfere with transitions from other peptides; and

(iv) represent transitions due to breakage of peptide bond at different sites of the protein.

4. The assay according to claim 1, wherein the peptides do not include any peptide that is bounded by KK, KR, RK or RR, either upstream of downstream in the corresponding protein sequence.

5. The assay according to claim 1, wherein each peptide of said set of peptides is unique to the corresponding protein.

6. The assay according to claim 1, wherein the peptides do not include peptides which were observed in post-translational modified forms.

7. The assay according to claim 1, wherein each set of peptides is prioritized according to one or more of the following ordered set of criteria:

(a) unique peptides first, then non-unique;

(b) peptides with no observed post-translational modifications first, then those observed with post-translational modifications;

(c) peptides within the mass range 800-3500 Da first, then those outside of 800-3500 Da; and

(d) sorted by decreasing number of variant residues.

8. The assay according to claim 7, wherein each set of peptides is prioritized according to all of the ordered set of criteria.

9. The assay according to any one of claim 7 or 8, wherein each prioritized set of peptides contains 1-5 peptides.

10. The assay according to any one of claims 1-9, wherein the two best peptides per protein and the two best transitions per peptide are selected based on experimental data resulting from LC-SRM-MS analysis of one or more of the following experimental samples: a biological disease sample, a biological control sample, and a mixture of synthetic peptides of interest.

11. The assay according to claim 10, wherein the biological disease and biological control samples are processed using an immunodepletion method prior to LC-SRM-MS analysis.

12. The assay according to claim 11, wherein the experimental samples contain internal standard peptides.

13. The assay according to claim 11, wherein the LC-SRM-MS analysis method specifies a maximum of 7000 transitions, including transitions of the internal standard peptides and transitions.

14. The assay according to claim 1, wherein the top two transitions per peptide are selected according to one or more of the following criteria:

(1) the transitions exhibit the largest peak areas measured in either of the two biological experimental samples;

(2) the transitions are not interfered with by other ions;

(3) the transitions do not exhibit an elution profile that visually differs from those of other transitions of the same peptide;

(4) the transitions are not beyond the detection limit of both of the two biological experimental samples; and

(5) the transitions do not exhibit interferences.

15. The assay according to claim 1, wherein the top two peptides per protein are selected according to one or more of the following criteria:

(1) one or more peptides exhibit two transitions according to claim 12 and represent the largest combined peak areas of the two transitions according to claims 12; and

(2) one or more peptides exhibit one transition according to claim 12 and represent the largest combined peak areas of the two transitions according to claim 12.

16. An assay developed according to the method of claim 1.