Your search keyword '"Patel E"' showing total 5 results

1. Peptide Imaging: Maximizing Peptide Yield, Optimization of the "Peptide Mass Fingerprint".

Author

Patel E

Subjects

Detergents chemistry, Peptide Mapping, Proteolysis, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization, Peptides chemistry, Proteomics methods

Abstract

In Matrix Assisted Laser Desorption Ionization Mass Spectrometry Imaging (MALDI-MSI), identification of observed proteins remains a challenge primarily due to the drop in sensitivity of time-of-flight (TOF) mass spectrometers beyond the mass range of 25-35 kDa (Francese et al. High Throughput Screen 12: 156-174, 2009) and inadequate mass resolving power at those molecular weights. To counteract this, a bottom-up proteomic approach is often employed. Proteolysis digests proteins into smaller peptide fragments, typically between 500 and 3000 Da which are easier to detect with a higher mass accuracy. Here, we describe the addition of a MS-compatible detergent to the endopeptidase trypsin, to enhance in situ proteolysis efficiency and peptide intensity.

Published

2017

2. Proteomics goes forensic: Detection and mapping of blood signatures in fingermarks.

Author

Deininger L, Patel E, Clench MR, Sears V, Sammon C, and Francese S

Subjects

Humans, Trypsin chemistry, Biomarkers blood, Forensic Genetics methods, Proteomics, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization methods

Abstract

A bottom up in situ proteomic method has been developed enabling the mapping of multiple blood signatures on the intact ridges of blood fingermarks by Matrix Assisted Laser Desorption Mass Spectrometry Imaging (MALDI-MSI). This method, at a proof of concept stage, builds upon recently published work demonstrating the opportunity to profile and identify multiple blood signatures in bloodstains via a bottom up proteomic approach. The present protocol addresses the limitation of the previously developed profiling method with respect to destructivity; destructivity should be avoided for evidence such as blood fingermarks, where the ridge detail must be preserved in order to provide the associative link between the biometric information and the events of bloodshed. Using a blood mark reference model, trypsin concentration and spraying conditions have been optimised within the technical constraints of the depositor eventually employed; the application of MALDI-MSI and Ion Mobility MS have enabled the detection, confirmation and visualisation of blood signatures directly onto the ridge pattern. These results are to be considered a first insight into a method eventually informing investigations (and judicial debates) of violent crimes in which the reliable and non-destructive detection and mapping of blood in fingermarks is paramount to reconstruct the events of bloodshed., (© 2016 WILEY-VCH Verlag GmbH & Co. KGaA, Weinheim.)

Published

2016

3. A proteomic approach for the rapid, multi-informative and reliable identification of blood.

Author

Patel E, Cicatiello P, Deininger L, Clench MR, Marino G, Giardina P, Langenburg G, West A, Marshall P, Sears V, and Francese S

Subjects

Amino Acid Sequence, Animals, Blood Stains, Child, Horses, Humans, Proteolysis, Reproducibility of Results, Time Factors, Blood, Forensic Medicine methods, Proteomics methods

Abstract

Blood evidence is frequently encountered at the scene of violent crimes and can provide valuable intelligence in the forensic investigation of serious offences. Because many of the current enhancement methods used by crime scene investigators are presumptive, the visualisation of blood is not always reliable nor does it bear additional information. In the work presented here, two methods employing a shotgun bottom up proteomic approach for the detection of blood are reported; the developed protocols employ both an in solution digestion method and a recently proposed procedure involving immobilization of trypsin on hydrophobin Vmh2 coated MALDI sample plate. The methods are complementary as whilst one yields more identifiable proteins (as biomolecular signatures), the other is extremely rapid (5 minutes). Additionally, data demonstrate the opportunity to discriminate blood provenance even when two different blood sources are present in a mixture. This approach is also suitable for old bloodstains which had been previously chemically enhanced, as experiments conducted on a 9-year-old bloodstain deposited on a ceramic tile demonstrate.

Published

2016

4. Alternative surfactants for improved efficiency of in situ tryptic proteolysis of fingermarks.

Author

Patel E, Clench MR, West A, Marshall PS, Marshall N, and Francese S

Subjects

Amino Acid Sequence, Animals, Molecular Sequence Data, Peptides metabolism, Proteins metabolism, Proteolysis, Rats, Trypsin metabolism, Brain Chemistry, Peptides analysis, Proteins analysis, Proteomics methods, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization methods, Surface-Active Agents chemistry

Abstract

Despite recent improvements to in situ proteolysis strategies, a higher efficiency is still needed to increase both the number of peptides detected and the associated ion intensity, leading to a complete and reliable set of biomarkers for diagnostic or prognostic purposes. In the study presented here, an extract of a systematic study is illustrated investigating a range of surfactants assisting trypsin proteolytic activity. Method development was trialled on fingermarks; this specimen results from a transfer of sweat from an individual's fingertip to a surface upon contact. As sweat carries a plethora of biomolecules, including peptides and proteins, fingermarks are, potentially, a very valuable specimen for non-invasive prognostic or diagnostic screening. A recent study has demonstrated the opportunity to quickly detect peptides and small proteins in fingermarks using Matrix Assisted Laser Desorption Ionization Mass Spectrometry Profiling (MALDI MSP). However, intact detection bears low sensitivity and does not allow species identification; therefore, a shotgun proteomic approach was employed involving in situ proteolysis. Data demonstrate that in fingermarks, further improvements to the existing method can be achieved using MEGA-8 as surfactant in higher percentages as well as combinations of different detergents. Also, for the first time, Rapigest SF, normally used in solution digestions, has been shown to successfully work also for in situ proteolysis.

Published

2015

5. A proteomic approach for the rapid, multi-informative and reliable identification of blood

Author

Vaughn G. Sears, Andrew West, Malcolm R. Clench, Paola Cicatiello, Glenn Langenburg, Peter S. Marshall, Lisa Deininger, Gennaro Marino, Simona Francese, Ekta Patel, Paola Giardina, Patel, E., Cicatiello, Paola, Deininger, L., Clench, M. R., Marino, G., Giardina, Paola, Langenburg, G., West, A., Marshall, P., Sears, V., and Francese, S.

Subjects

Proteomics, Time Factors, Computer science, Sample (material), Blood Stains, Analytical chemistry, 01 natural sciences, Biochemistry, Analytical Chemistry, 03 medical and health sciences, 0302 clinical medicine, Electrochemistry, Animals, Humans, Environmental Chemistry, Crime scene, Amino Acid Sequence, Horses, 030216 legal & forensic medicine, Child, Spectroscopy, business.industry, 010401 analytical chemistry, Reproducibility of Results, Pattern recognition, Forensic Medicine, 0104 chemical sciences, Identification (information), Blood, Proteolysis, Artificial intelligence, business

Abstract

Blood evidence is frequently encountered at the scene of violent crimes and can provide valuable intelligence\ud in the forensic investigation of serious offences. Because many of the current enhancement\ud methods used by crime scene investigators are presumptive, the visualisation of blood is not always\ud reliable nor does it bear additional information. In the work presented here, two methods employing a\ud shotgun bottom up proteomic approach for the detection of blood are reported; the developed protocols\ud employ both an in solution digestion method and a recently proposed procedure involving immobilization\ud of trypsin on hydrophobin Vmh2 coated MALDI sample plate. The methods are complementary as whilst one yields more identifiable proteins (as biomolecular signatures), the other is extremely rapid (5 minutes).\ud Additionally, data demonstrate the opportunity to discriminate blood provenance even when two different blood sources are present in a mixture. This approach is also suitable for old bloodstains which had been previously chemically enhanced, as experiments conducted on a 9-year-old bloodstain deposited on a ceramic tile demonstrate.

Published

2016