Patent Application
20220082576
The invention relates to a biochemical diagnostic test performed on peripheral blood, which allows the diagnosis of Attention Deficit Hyperactivity Disorder (ADHD). Specifically, the serum levels of at least 6 markers corresponding to 2 groups of functional lipids, esfingolipids and long-chain polyunsaturated fatty acids (LC-PUFAs) are measured, detecting a variation in concentrations with respect to the values of the control population.
ADHD is the most common neuro-psychiatric disorder in childhood, with global prevalences between 5-10%. The last decade has seen a marked increase in the diagnosis of ADHD and in the use of pharmacological treatment, which doubled between 2004 and 2015 (Davidovitch et al. BMC Pediatrics, 2017. 17:218). Since ADHD affects key areas in a child's intellectual, emotional, and relational development, the disorder is associated with a significant worsening in quality of life (Coghill et al. Eur Child Adolesc Psychiatry, 2017. 26:1283-1307).
Timely diagnosis and treatment of ADHD improves the patient's quality of life and mitigates the emotional and social impact of the disorder. However, pharmacological treatment is associated with increased cardiovascular risk (Shin et al. BMJ. 2016; 353: i2550.), therefore, diagnostic certainty is essential to assess the need for treatment. Currently, this diagnosis is exclusively clinical and based on the objectification of symptoms that meet the criteria established by consensus (DSM-5 or ICD-10), which require the doctor to assess the impact of the clinical picture on the social, school and emotional life of the child; an extremely difficult task in the context of medical consultations of an average duration between 15 and 30 minutes worldwide. Additionally, physicians face high comorbidity and clinical variability, which confuses diagnosis, and variability in symptomatic assessment from different reporting sources (McKeown et al. J Am Acad Child Adolesc Psychiatry, 2015 54(1): 53-6). All of this makes diagnosing ADHD a major clinical challenge, requiring in most cases several evaluations by a well-trained physician. Currently the gold standard for the diagnosis of this disorder is the clinical diagnosis made by a doctor specializing in child neurology/psychiatry, supported by neuropsychological studies that—although they have a very limited diagnostic value—help to characterize the specific cognitive profile for the patient and to rule out other alterations.
In this way the diagnosis of ADHD is exclusively clinical and does NOT have the diagnostic support of any objective tool. There is no specific neuropsychological profile for ADHD, so the application of batteries of neurocognitive tests has limited diagnostic utility. Having an objective diagnostic tool for ADHD would simplify and shorten the diagnostic process, reduce diagnostic errors and improve adherence to treatment.
So far, attempts to have an objective diagnostic tool for ADHD have focused mostly on the development of neuro-imaging-based detection algorithms, which have achieved sensitivities and specificities that rarely exceed 80% (Uddin et al. Trans) Psychiatry, 2017; 7, e1218). Although some of these methods show promising results, their clinical applicability is limited in children with ADHD, due to the low acceptability of the technique in these patients (Yerys et al. Hum Brain Mapp, 2009; 30:3426-3435). Additionally, extending the use of neuroimaging to isolated regions or large patient populations (as in a screening) is technically and economically difficult. The use of electro-encephalographic markers for the detection of ADHD has also been explored, with good results, the main limitation of these techniques being the low reproducibility of some of the analyses used (for example, ERPs; Kompatsiari et al. Neuroscience Letters, 2016; 617: 166-172).
Some groups of researchers, including one from the medical school of Universidad Católica de Chile, have reported algorithms based on the characterization of eye movements or pupillary size (Varela Casal et al. Journal of Attention Disorders, 2018; 1-16; Wainstein et al, Scientific Reports, 2017; 7: 8228). The use of these latter algorithms is attractive since they do not require invasive procedures and their implementation is low cost, but they need specific equipment, which limits their widespread application.
Previously, some research groups have explored the use of biochemical markers for the diagnosis of ADHD, for example Vogel et al. (Psychoneuro-endocrinology, 2017; 79:31-39), Alassehirli et al (The International Journal of Psychiatry in Medicine, 2015; 50(2): 238-247) and Percinel et al. (Child Psychiatry Hum Dev, 2016; 47:259-269), however its results are not very replicable and none has achieved the levels of sensitivity and specificity of those obtained by the method of this invention.
The need therefore persists for an objective analytical diagnostic test of easy implementation and interpretation that is a tool to support the current clinical diagnosis.
The inventors have met this need by developing a biochemical diagnostic test which, surprisingly, allows the diagnosis of Attention Deficit Hyperactivity Disorder by analyzing peripheral blood of patients.
The invention aims at a biochemical diagnostic test performed on peripheral blood, which allows the diagnosis of Attention Deficit Hyperactivity Disorder (ADHD), with sensitivity of 93% and specificity of 84% or higher according to pilot results. The sensitivity and specificity indicated were evaluated in relation to a gold standard compound, widely used in research, comprising the clinical diagnosis and the positive response of the patient to the specific pharmacological treatment of the disease.
The biochemical test of the invention is based on the analysis of serum levels of at least 6 markers, corresponding to 2 groups of functional lipids, sphingolipids and long-chain polyunsaturated fatty acids (LC-PUFAs), detecting a variation in the concentrations of said markers with respect to the values for the control population. Specifically, the markers used are the sphingolipids Ceramide C16:0, Ceramide C24:0, Deoxy dihydro-ceramide C24:1 and Sphinganine 1-phosphate and the LC-PUFAs docosahexaenoic acid (DHA) and eicosapentaenoic acid (EPA).
The invention comprises 2 consecutive phases: a first phase of analytical processing and a second phase of statistical processing. In the first phase, serum levels of at least 6 markers corresponding to 2 groups of functional lipids, sphingolipids and long-chain polyunsaturated fatty acids (LC-PUFAs) are measured, and up to 28 functional lipid markers can be measured, which would contribute to obtaining greater specificity in the results while maintaining predictive quality. In a preferred embodiment, where the minimum of markers is selected to achieve diagnostic accuracy, the preferred markers used are the sphingolipids Ceramide C16:0, Ceramide C24:0, Deoxy dihydro-ceramide C24:1 and Sphinganine 1-phosphate and Ic-PUFAs docosahexaenoic acid (DHA) and eicosapentaenoic acid (EPA).
The markers are measured preferably in serum obtained by centrifugation of a peripheral blood sample collected in a tube without anticoagulant, by LC-MSMS after lipid extraction, in the case of sphingolipids, or by GC-MS after extraction and derivatization of lipids, in the case of LC-PUFAs. Both technologies are considered the gold standard for the analytical determination of each group of markers.
In the second phase, whether patients are positive or negative for ADHD is determined using a predictive algorithm developed by the inventors that receives as input variables the serum levels of the indicated markers, normalizes the data and confers a total score to each sample, which is submitted to a critical decision point to obtain the classification. Depending on the selected markers, the absolute value of each marker or a ratio between two markers will be used. Due to its high sensitivity, the most appropriate use of this test is diagnostic screening.
The method, as indicated, is based on the joint determination of at least 6 lipid markers, which are used as input variables for a predictive algorithm. The joint use of these markers to give greater sensitivity and specificity to ADHD discrimination is new and not obvious, given that no significant differences in ADHD have been reported for some of them, such as sphinganine 1-phosphate. This reveals that the relative balance of the levels of these markers—and not their absolute level—gives the discriminating power to the method of the invention.
Optionally the method can use as input variables up to 28 lipid markers, selected from from sphinganin-1-phosphate, sphingosine-1-phosphate, ceramides C16:0, C18:0, C20:0, C22:0, C24:0 and C24:1; dihidroceramides C18, C18:1, C24:0 and C24:1; deoxi-ceramides C16:0 and C24:1 and deoxi-dihidroceramides C16:0 and C24:1; sphingomyelins (SM) SM C16:0, SM C18:0, SM C18:1 and SM C24:1, linoleic acid (LA), γ-linoleic acid (GLA), alpha-linolenic acid (ALA), dihomo-gamalinolenic acid (DGLA), arachidonic acid (AA), eicosapentaenoic acid (EPA), docosapentanoic acidor (DPA), docosahexaenoic acid (DHA).
In the case of opting for a complex diagnostic test, with a greater number of variables, the classification model obtained demonstrated a sensitivity of 93% and a specificity of 96% in the training procedure of the predictive algorithm and a sensitivity of 100% and specificity of 83% during the validation procedure of the predictive algorithm.
So far there is no validated tool that fulfills the function of the method proposed by this invention. There are publications of algorithms based on neuroimaging (NMR) and EEG for the detection of ADHD, which—in general—do not present sensitivities/specificities greater than 80% and show little analytical reproducibility, in addition to the complexity of implementation. Since the analytical phase of our diagnostic test is performed using techniques that constitute the gold standard for each group of molecules, the analytical imprecision associated with it is the least possible with current technology (in general less than 10% inter-run). Finally, the use of a peripheral biological sample, minimally invasive and easy to store and transport, gives this test comparative advantages in relation to NMR or EEG for widespread use, for example, as a screening tool.
Recently the inventors published for the first time the significant decrease of specific sphingolipids in children with ADHD (especially sphingomyelins and long-chain ceramides) and raised the importance of this group of functional lipids as an eventual biomarker and/or pathogenic factor for ADHD. These results are based on a pilot study that characterized the serum levels of 20 molecular species of sphingolipids in 90 subjects, including patients with ADHD and 2 control groups: a) first-degree relatives without diagnosis of ADHD who live and share their main meal with the index case and b) controls without ADHD and without family history of the disease. This pilot study described that low serum levels of total sphingomyelines present a sensitivity of 79% and specificity of 80% for the diagnosis of ADHD (Henriquez-Henriquez et al. Front. Neurosci, 2015. 9:300).
In a subsequent analysis of the data obtained, the inventors were discriminating the markers that correlate with the development of ADHD, finding that the combination of markers of the 2 lipid families (sphingolipids and LC-PUFAs) are able to discriminate patients with ADHD more efficiently than that reported by the same group in the pilot study. The results of the analysis of ROC on the classification achieved by the method of the invention demonstrate that it is able to discriminate patients with ADHD with a sensitivity and specificity much higher than that reported in the previous publication (sensitivity 93%, specificity 84%).
For the expert in the technique, it will be evident that each of the markers can be detected with any method available in the technique, as the method of the invention correlates the variation of normal values with the presence of attention deficit and hyperactivity disorder. For this reason, the invention can be applied independently of the technique by which the concentration of the selected lipids is determined and regardless of the number of markers used. All these embodiments are considered within the scope of the present invention.
Thus, as indicated by the in vitro diagnostic method for Attention Deficit Hyperactivity Disorder (ADHD) comprises a first phase of analic measurement from a peripheral blood sample of the markers selected from 2 groups of functional lipids: sphingolipids and long-chain polyunsaturated fatty acids (LC-PUFAs) and a second statistical phase where the normalized value for each marker is determined, assigning a total score to the sample using a predictive model and classifying it as positive or negative for ADHD if said total score exceeds an established value.
The markers selected in the first phase correspond to at least 6 functional lipids to achieve diagnostic accuracy, and up to 28 markers can be measured to obtain a greater sensitivity/specificity in the results. Depending on the set of markers used, the variables to be evaluated may be absolute values and/or a ratio between markers.
In the preferred embodiment of the invention, the 6 markers determined in the first stage determine 4 variables for the statistical phase, since 4 of them are analyzed as ratios.
The score is assigned by calculating the z-score for each variable analyzed, considering as an average value the amount obtained for the control population without ADHD determined according to clinical criteria (gold standard). The z-score obtained for each marker or marker ratio is used as an input variable in the predictive model that will determine the score.
A sample will be considered ADHD positive if the score obtained in the predictive algorithm is less than an established value of critical decision, or in other words if there is a minimum set of differences in the variables analyzed with respect to the normal values obtained in the control group for these same variables.
In the case of the measurement of 6 markers for the use of 4 variables (see
Where the critical difference is determined in relation to the score assigned by a predictive algorithm, which will relate the existence/non-existence of these variations in the studied sample with respect to the normal values obtained in the control group. And where the critical decision point is established by correlating the values obtained in samples of patients without ADHD and samples of patients with ADHD, for a given population.
This can be done with the 4 variables corresponding to the 6 main markers, and optionally with one or more of these 22 markers: sphingosine-1-phosphate, ceramides C18:0, C20:0, C22:0 and C24:1; dihydroceramides C18, C18:1, C24:0 and C24:1; deoxy-ceramides C16:0 and C24:1 and deoxy-dihydroceramide C16:0; sphingomyelins (SM) SM C16:0, SM C18:0, SM C18:1 and SM C24:1, linoleic acid (LA), γ-linoleic acid (GLA), alpha-linolenic acid (ALA), dihomo-gamalinolenic acid (DGLA) arachidonic acid (AA), and docosapentanoic acid (DPA), In one embodiment, the 28 markers are studied.
In the case of using the optional method with 7 or up to 28 markers, once the serum values of each one have been determined, a correlation is made between the variation of serum concentrations and the clinical diagnosis of ADHD. This assigns a score to even small differences in a set of variables. Thus, a sample is generally considered as ADHD positive if the score obtained in a predictive algorithm differs from the established value of critical decision, where the algorithm determines the minimum conditions for the classification to be positive. These 22 markers can be evaluated by their absolute values or as ratios between 2 of them, for a pair of markers.
The predictive algorithm can be developed using various analytical tools, including mathematical or statistical modeling and machine learning (neural networks, etc.).
Next, a preferred mode of embodiments of the invention is exemplified, without limiting the technical variants that an expert in the field can incorporate or modify, and that are within the scope of the inventive concept that we protect in this invention.
1.1 Blood Sample Collection and Pre-Analytical Processing.
The sample is obtained by peripheral venous puncture, with minimum fasting of 4 hrs, in a tube without anticoagulant. In the laboratory the sample is centrifuged to obtain serum, which passes to the analysis phase.
1.2 Measurement of Lipidomic Markers.
For the analysis of sphingolypical markers, serum lipids are extracted, using a technique standardized in our laboratory and widely validated by the literature (Folch's modified method, Folch J., Lees M., Sloane-Stanley G. H. A simple method for the isolation and purification of total lipids from animal tissues. J. Biol. Chem. 1957; 226:497-509). Sphingolipids are then detected and quantified using a previously standardized protocol on a liquid chromatography—LC-MS/MS mass spectrometry platform. For the analysis of the markers corresponding to LC-PUFAs, the serum lipids are extracted and derivatized by protocol and the LC-PUFAs are detected and quantified by means of a standardized protocol in gas chromatography—GC-MS mass spectrometry platform. The analytical features of this last protocol have been published by our laboratory (Henriquez-Henriquez et al. ω-3 Long-Chain Polyunsaturated Fatty Acids and Fatty Acid Desaturase Activity Ratios as Eventual Endophenotypes for ADHD. J Atten Disord. 2015 November; 19(11):977-86.doi: 10. 1177/1087054712461175)
1.3 Application of the Classificatory Model.
In the second phase, a predictive model receives as input variables the serum levels of the 6 markers indicated, either as an absolute marker or as a ratio (absolute value for Deoxy dihydro-ceramide C24:1 and Sphinganin 1-P and ratio C24:0/C16:0 and DHA/EPA). The method was validated considering training and validation data, and then proceeded to execute the classification with each of the samples included in the study data. Through an algorithm, each sample is assigned a total score or score, which is subjected to a critical decision point to obtain the classification that allows determination of whether the sample is positive or negative for ADHD.
The differences that exist for the different analytes of patients with ADHD and the healthy population, without this disorder, were determined. The inventors found that there are differences between the serum concentrations of Deoxy dihydro-ceramide C24:1 and Sphinganin 1-P between the two groups and that the difference between the ratios of Ceramide C24:0/Ceramide C16:0 is also relevant (C24:0/C16:0) and DHA/EPA. The results are shown in
The serum values of the markers of the invention were analyzed in samples from 11 patients, between 7 and 17 years of age, 6 of them with clinical diagnosis of ADHD and 5 healthy controls. A correlation was made between the variation of serum concentrations of Ceramide C16:0, Ceramide C24:0, Deoxy dihydro-ceramide C24:1, Sphinganin 1-phosphate, docosahexaenoic acid (DHA) and eicosapentaenoic acid (EPA) and the clinical diagnosis of ADHD.
The results are shown in Table 1, which details the absolute levels obtained in peripheral blood for the 6 analytes considered in the invention, and the value of the score or score assigned by its variation, of the analyte itself for Deoxy dihydro-ceramide C24:1 and Sphinganin 1-P or the ratios already indicated, C24:0/C16:0 and DHA/EPA. The cut-off point (or critical decision point) was designated in the score 0.5, where a score less than or equal to 0.5 is indicative of ADHD, and a score greater than 0.5 is indicative of the absence of the disease. In these 11 cases chosen at random, the method of the invention had a concordance of 82% (9 of 11) with the composite diagnosis or gold standard.
In this table Deoxy dihydro-ceramide C24:1 is identified as DeoxyC24:1DH, Sphinganin 1-P is identified as Sa1p., Ceramide C16:0 is identified as C16, Ceramide C24:0 is identified as C24, docosahexaenoic acid is identified as DHA and eicosapentaenoic acid is identified as EPA.
In the analyzed data it can be seen that there were 2 cases where one of the lipids, specifically Sphinganine 1-P (Sa1p) was not determined. As the method of the invention weights the different variations of the 6 analytes, it is possible to use it even without one of them, and as you can see in the results, the method maintains its diagnostic predictive value.
The serum values of the markers of the invention were analyzed in samples from 77 patients, 28 of them with clinical diagnosis of ADHD and 49 healthy controls. A correlation was made between the variation of serum concentrations of Ceramide C16:0, Ceramide C24:0, Deoxy dihydro-ceramide C24:1, Sphinganin 1-phosphate, docosahexaenoic acid (DHA) and eicosapentaenoic acid (EPA) and the clinical diagnosis of ADHD. The results are shown in
These results demonstrate the great usefulness of the test of the invention as an objective tool for the diagnosis of ADHD.
| Filing Document | Filing Date | Country | Kind |
|---|---|---|---|
| PCT/CL2019/050002 | 1/3/2019 | WO | 00 |
