A filter represents a question and the customized view is designed to display information required to make a rapid yes/no answer to violations in the selected sample. The filter in Figure 4 ensures that only confident matches are displayed. This filter restricts the viewed target list matches to those that are within a retention time tolerance of ±0.5 minutes, that have a mass accuracy within ±6ppm, that have a response over 300 and that match at least one target fragment ion. False detections are avoided due to the specificity of requiring an accurate mass fragment ion in addition to matching the tighter criteria set for retention time, mass accuracy and intensity in the filter compared to the analysis method.
A “view” containing the component summary, mass spectra and extracted ion chromatograms was designed to display all of the information required to rapidly verify the confident matches in this workflow step. From Figure 5 we can see the wealth of information available for the match of thiacloprid in the dried cherry sample. In the component summary (Figure 5A) we see that the compound has been matched within 0.06 minutes of the expected retention time, a mass error of 0.82 ppm and an expected accurate mass fragment was matched from the target list. In addition, four accurate mass fragments have been identified by the Fragment Match tool, which automatically interrogates the high energy data once a target match is made. A low isotope score for m/z and intensity gives confidence that the component isotope pattern closely matches that of the compounds theoretical isotopic pattern.
Data componentization is key to the success of UNIFI data review since all of the mass spectral data displayed for a match are from a tight retention time band at the apex of the chromatographic peak. This also results in cleaner looking spectra compared to a conventional background subtracted spectra from an extracted ion chromatogram, as can be seen in figure 5B. The isotope scores in the component summary are based on the entire cluster in the green shaded area for the most intense adduct (H+ in this case).
The high energy data shows fragment ion information and two example fragment ion identifications are highlighted in figure 5C. The fragment ions matched from those in the Scientific Library are automatically annotated with the mass error. Fragment ions matched by the Fragment Match tool are automatically annotated with the proposed structure and mass error from the theoretically calculated mass. All isotopic information is obtained for fragments in addition to precursors, which is especially useful for atoms with characteristic isotopic patterns, such as the halogens. In the thiacloprid example, the expected fragment formula contains a chlorine atom. The measured isotopic pattern of the high energy fragment agrees with the theoretical distribution for the presence of a single chorine atom. This increases confidence in the compound match.
The final piece of evidence pointing to a confident match lies in the Chromatogram window. Extracted ion chromatograms (Figure 5D) are displayed for precursor ions and matched fragment ions. The peak shape and apex retention time should be identical for a precursor and its fragments, as can be seen for thiacloprid in Figure 5D.
Using the workflow step for confident matches, a user can verify these matches within seconds. Componentization of data makes all of this possible. Any false detects matched using a wide tolerance of retention time and mass error are automatically filtered out from this view, vastly improving efficiency of data interpretation without the risk of introducing false negatives in the data processing step.
