Human monitoring analysis calculation
Human monitoring analysis computes substance concentration estimates for a biological matrix (e.g., urine or blood) based on human monitoring data. These estimates are specified at the level of long term average concentrations for individuals in case of chronic assessments, or concentrations for individual-days in case of acute assessments. The concentrations are computed independently for each substance and biological matrix.
The main steps, and also performed in this order, for computing human monitoring concentration estimates are:
Imputation of censored values.
Imputation of missing values.
Standardise blood for lipid content.
Standardise/normalise urine for creatinine or specific gravity.
Apply conversion of substance concentrations from other biological matrices.
Calculation of individual concentrations (chronic) or individual day concentrations (acute).
Imputation of censored values
Similar to concentrations measurements in food, human monitoring measurements contain measurements below the limit of reporting and similar to concentrations modelling in foods, human monitoring analysis addresses these censored values and replaces them with imputed concentration values. Two approaches are available:
Impute using a non-detects handling method.
Impute using a draw from the left tail of the censored lognormal distribution. See also concentration models and concentration model types.
The available non-detects handling methods for deterministic imputation are:
Replace censored values by zero.
Replace censored values by a factor * LOR, the factor is set between zero and one.
Replace non-detects by a factor * LOD and non-quantifications by LOD + factor * (LOQ - LOD), the factor is set between zero and one.
Note that for the option based on the censored lognormal distribution also a non-detects handling method needs to be specified. Occasionally, fitting the censored lognormal model fails and the deterministic imputation method is used as fallback.
In Figure 83, the human monitoring concentrations data for three bisphenols are imputed with a factor * LOR and the summary statistics are visualized.
Imputation of missing values
For missing concentration measurements, three imputation methods are available. The third opion ignores imputation and all missing values remain in the data set.
Replace missing values by zero.
For each substance and combination of biological matrix and sampling type, replace missing values by a random draw from the non-missing concentration values (samples). This is conditional on the specified minimum percentage of non-missing values.
Do not impute missing values
Imputation of missing values by a random draw from the data is conditional on the specified percentage of non-missing values. When the percentage of non-missing values for a specific substance and combination of biological matrix and sampling type in the data is smaller than the specified percentage, imputation is ignored. This is to prevent that imputation takes place using a set of imputation values that is not representative or unrealistically small (e.g. one or a few values). Note that for the second imputation method, more refined methods could be used. E.g., when for a given day multiple samples are available and one is missing, then this sample might be neglected in the computation of an average exposure. Also, when samples have been taken at different time-slots, impute the missing records using samples from the same time-slot.
Standardise blood for lipid content
Lipid-soluble substances measured in blood data are typically standardised by total lipid content. Three methods are in available, namely:
Standardisation based on gravimatic analysis.
Standardisation based on enzymatic summation analysis.
Standardisation based on Bernert et al. (2007), total lipids (mg/dL) = 2.27 * total cholesterol + triglycerides + 62.3 mg/dL.
The standardisation is only applied to lipid-soluble substances, see Substances data formats. After standardisation, the amount of substance is expressed per g lipid e.g. \(\mu g / g \, {\small \mathtt{lipid}}\). Note that substance concentrations in blood samples with unmeasured lipid concentrations are set to missing after specifying option blood standardisation.
Standardise/normalise urine for creatinine or specific gravity
Two methods are available for correcting spot urine measurements for creatinine of specific gravity.
Normalisation based on specific gravity.
Standardisation based on creatinine content.
Urine’s specific gravity is determined by the concentration of excreted molecules in the urine. In adult humans, normal specific gravity values range from 1.010 to 1.030. The specific gravity normalisation used here is equal to \((1.024 - 1) / (specific \, gravity - 1)\). The specific gravity value should be available in the HBM data, otherwise urine sample concentrations are set to missing.
After standardisation for creatinine content, the amount of substance is expressed per g creatinine e.g. \(\mu g / g \, {\small \mathtt{creatinine}}\). Note that substance concentrations in urine samples where the creatinine content is not measured are set to missing values after specifying option urine standardisation.
Apply conversion of substance concentrations from other biological matrices
Conversion of substances measured in biological matrices other than the target matrix is used when the number of substances in the target biological matrix is limited. For instance, in target matrix urine (spot) five substances are measured. For the same individuals also the blood (serum) concentrations are analysed resulting in a additional set of concentrations for five different substances. These five substances from blood (source matrix) are converted to the target matrix urine by checking the option Apply conversion of substance concentrations from other biological matrices and specifying the ‘between matrix conversion’ multiplication factor. Then, the analysis continues with ten substances. Conversion of substance concentrations is performed after imputation of censored and missing values. Selecting specific substances for conversion is possible through the selection options in the primary entity substances module.
Note that after choosing Do not impute missing values or Impute from data, missing value imputation, the data still contains missing values. These values may be imputed from other substance concentrations after applying matrix conversion.
Restricting the monitoring concentrations
After imputation of non-detects and missing values, standardisation/normalisation, eventually followed by conversion of substance concentrations from other biological matrices, some individual day monitoring concentration may contain missing values (e.g. after ‘Do not impute missing values or Impute from data, missing value imputation). All individual day samples with missing values for one or more substances are removed from the data set and the analysis continues.
Calculation of acute human monitoring concentrations
For acute assessments, the monitoring concentrations are computed for each substance and biological matrix as average individual-day concentrations. The computation is done after imputation of censored and missing values, eventually followed by a conversion of substance concentrations from other biological matrices. For a given substance and biological matrix, the acute individual-day concentration \(c_{ij}\) for individual \(i\) on day \(j\) is:
where \(n_{\mathtt{samples}}\) is the number of samples available for individual \(i\) on day \(j\), and \(c_{ijk}\) the concentration of the \(k\)-th sample of the individual day \(j\).
After urine normalisation for specific gravity:
where \(\mathit{sg}\) denotes the specific gravity correction factor for that individual day.
After standardisation for blood lipid content:
- . math::
c’_{ij} / g , {small mathtt{lipid}} = frac{c_{ij}} { c_{ij} , {small mathtt{lipid}}}
where \(\mathit{c'_{ij}}\) denotes the lipid concentration per \({ g \, \small \mathtt{lipid}}\). The standardisation is only performed for lipid soluble substances. After standardisation the concentration of the substance is is expressed as substance amount, with an user specified unit, per \({ g \, \small \mathtt{lipid}}\).
The standardisation for creatinine is similar to the above equation replacing \({\small \mathtt{lipid}}\) by \({\small \mathtt{creatinine}}\).
Calculation of chronic human monitoring concentrations
For chronic assessments, the monitoring concentrations are computed as the average monitoring concentrations of multiple individual-days for each substance and biological matrix. The computation is done after imputation of censored and missing values, eventually followed by a conversion of substance concentrations from other biological matrices. The chronic concentration \(c_{i}\) for individual \(i\) is computed as:
where \(n_{\mathtt{days}}\) is the number of days that individual \(i\) was monitored, and \(c_{ij}\) denotes the average monitoring concentration of individual \(i\) on day \(j\).
Standardisation and normalisation of blood and urine samples respectively, are similar to the expressions for the calculation of individual day concentrations (acute).