Your search keyword '"Solomon Park"' showing total 6 results

1. Volumetric Assessment of Pediatric Vascular Malformations Using a Rapid, Hand-Held Three-Dimensional Imaging System.

Author

Ethan J. Speir, C. Matthew Hawkins, Michael J. Weiler, Michael Briones, Rachel Swerdlin, Solomon Park, and J. Brandon Dixon

Published

2019

2. Volumetric Assessment of Pediatric Vascular Malformations Using a Rapid, Hand-Held Three-Dimensional Imaging System

Author

Rachel Swerdlin, M. Weiler, Solomon Park, C. Matthew Hawkins, J. Brandon Dixon, Michael Briones, and Ethan J. Speir

Subjects

Male, Percutaneous, Adolescent, Infrared Rays, Vascular Malformations, Point-of-Care Systems, Sedation, 3d scanning, Article, 030218 nuclear medicine & medical imaging, Young Adult, 03 medical and health sciences, Imaging, Three-Dimensional, 0302 clinical medicine, Image Interpretation, Computer-Assisted, Humans, Medicine, Volume reduction, Radiology, Nuclear Medicine and imaging, Child, Radiological and Ultrasound Technology, business.industry, Hand held, Vascular malformation, Infant, medicine.disease, Computer Science Applications, Three dimensional imaging, Child, Preschool, Female, medicine.symptom, business, Nuclear medicine, 030217 neurology & neurosurgery, Volume (compression)

Abstract

The effect of percutaneous, surgical, and medical therapies for vascular malformations (VMs) is often difficult to quantify volumetrically using cross-sectional imaging. Volumetric measurement is often estimated with serial, expensive MRI examinations which may require sedation or anesthesia. We aim to explore whether a portable 3D scanning device is capable of rapid, accurate volumetric analysis of pediatric VMs. Using an iPad-mounted infrared scanning device, 3D scans of patient faces, arms, and legs were acquired over an 8-month study period. Proprietary software was use to perform subsequent volumetric analysis. Of a total of 30 unilateral VMs involving either the face, arms, or legs, 26 (86.7%) VMs were correctly localized by discerning the larger volume of the affected side compared to the normal contralateral side. For patients with unilateral facial VMs (n = 10), volume discrepancy between normal and affected sides differed compared with normal controls (n = 19). This was true for both absolute (60 cc ± 55 vs 15 cc ± 8, p = 0.03) as well as relative (18.1% ± 13.2 vs 4.0% ± 2.1, p = 0.008) volume discrepancy. Following treatment, two patients experienced change in leg volume discrepancy ranging from − 17.3 to − 0.4%. Using a portable 3D scanning device, we were able to rapidly and noninvasively detect and quantify volume discrepancy resulting from VMs of the face, arms, and legs. Preliminary data suggests this technology can detect volume reduction of VMs in response to therapy. ELECTRONIC SUPPLEMENTARY MATERIAL: The online version of this article (10.1007/s10278-019-00183-6) contains supplementary material, which is available to authorized users.

Published

2019

3. An updated protocol based on CLSI document C37 for preparation of off-the-clot serum from individual units for use alone or to prepare commutable pooled serum reference materials.

Author

Danilenko U, Vesper HW, Myers GL, Clapshaw PA, Camara JE, and Miller WG

Subjects

Humans, Reference Values, Blood Chemical Analysis standards, Blood Specimen Collection methods, Documentation, Serum chemistry

Abstract

Manufacturers of in vitro diagnostic medical devices, clinical laboratories, research laboratories and calibration laboratories require commutable reference materials that can be used in the calibration hierarchies of medical laboratory measurement procedures used for human specimens to establish metrological traceability to higher order reference systems. Commutable materials are also useful in external quality assessment surveys. In order to achieve these goals, matrix-based reference materials with long-term stability, appropriate measurand concentrations and commutability with individual human specimens are required. The Clinical and Laboratory Standards Institute (CLSI) guideline C37-A (now archived) provided guidance to prepare commutable pooled serum reference materials for use in the calibration hierarchies of cholesterol measurement procedures. Experience using the C37-A guideline has identified a number of technical enhancements as well as applications to measurands other than cholesterol. This experience is incorporated into this updated protocol to ensure the procedure will continue to meet the needs of the medical laboratory. The updated protocol describes a procedure for preparing frozen human serum units or pools with minimal matrix alterations that are likely to be commutable with individual human serum samples. The protocol provides step-by-step guidance for the planning phase, collection of individual serum units, processing the units, qualifying the units for use in a pool and frozen storage of aliquots of pooled sera to manufacture frozen serum pools. Guidance on how to perform quality control of the final product and suggestions on documentation are also provided.

Published

2020

4. Role of normalization in the elimination of abundant myelin sequences in spinal cord cDNA libraries produced by suppression subtractive hybridization.

Author

Lathia KB, Yan Z, and Clapshaw PA

Subjects

Animals, Apoferritins genetics, Apoferritins metabolism, Base Sequence, Blotting, Northern, Expressed Sequence Tags, Gene Expression Regulation, Male, Mice, Mice, Inbred C57BL, Myelin Basic Protein genetics, Myelin Basic Protein metabolism, Myelin Proteolipid Protein genetics, Myelin Proteolipid Protein metabolism, Myelin Sheath metabolism, RNA, Messenger genetics, RNA, Messenger metabolism, Reverse Transcriptase Polymerase Chain Reaction, Visual Cortex metabolism, Gene Library, Myelin Sheath genetics, Nucleic Acid Hybridization methods, Spinal Cord metabolism

Abstract

Spinal cord libraries subtracted against visual cortex using suppression subtractive hybridization SSH are dominated by abundant gene sequences derived from myelin elements. We compared our subtracted library results of three of these abundant sequences to published expressed sequence tag libraries that are not normalized and not subtracted and presumed representatives of murine spinal cord mRNA abundance. We show that: all three abundant sequences, myelin basic protein (Mbp), proteolipid protein (Plp1) and Ferretin heavy chain (Fth1) are highly expressed in spinal cord when this structure is compared to visual cortex; myelin basic protein is represented in our subtracted libraries but at a low frequency, whereas Plp1 and Fth1 represent nearly one-third of all sequences in these libraries; mirror orientation selection, a procedure designed to reduce background sequences, generates libraries very similar in abundance to SSH; proteolipid protein can be reduced in these libraries by adding Plp1 sequences to the driver in the SSH procedure and also by subtracting Plp1 directly from tester and driver. We conclude that adequate normalization is essential to reduce the presence of abundant sequences in SSH libraries.

Published

2009

5. Murine spinal cord transcriptome analysis following reduction of prevalent myelin cDNA sequences.

Author

Yan Z, Lathia KB, and Clapshaw PA

Subjects

Animals, Base Sequence, Blotting, Northern, Gene Expression Regulation, Male, Mice, Mice, Inbred C57BL, Neuroglia metabolism, RNA, Messenger genetics, RNA, Messenger metabolism, DNA, Complementary genetics, Gene Expression Profiling, Myelin Sheath genetics, Spinal Cord metabolism

Abstract

From 1,000 randomly selected colonies from cDNA libraries derived from murine spinal cord subtracted against white matter by means of suppression subtractive hybridization, 220 clones were identified as differentially expressed by dot blot analysis. Sequence analysis by the BLAST programming identified 140 unique genes. (1) The percentage of known sequences from myelin and other glial sources was reduced by approximately 75% over previous, similar subtractions employing visual cortex as the driver. (2) Differentially expressed genes tended to reflect existing expectations concerning structure and function of the spinal cord. (3) About 35% of all genes differentially expressed in the spinal cord in this study are also known to be differentially expressed for this structure as tabulated in the UniGene database. (4) About 33% of all genes differentially expressed in the present study are recorded as not present when measured in the spinal cord according to the UniGene database indicating that present techniques are not recording about a third of differentially expressed genes in this structure. (5) About 15% of all differentially expressed genes are for unknown, putative or hypothetical protein products. (6) About 4% of all differentially expressed genes are novel expressed sequence tags for the mouse. The current study demonstrates the importance of reducing the presence of glial associated sequences when comparing brain regions. It is concluded that the persistence of some myelin sequences in the spinal cord when white matter is used as the driver indicates that myelination is more active in this structure than for those areas represented by white matter and corpus callosum.

Published

2009

6. Spinal cord transcriptome analysis using suppression subtractive hybridization and mirror orientation selection.

Author

Lathia KB, Yan Z, and Clapshaw PA

Subjects

Animals, Gene Expression Profiling, Gene Library, Male, Mice, Mice, Inbred C57BL, Myelin Sheath metabolism, Nerve Tissue Proteins genetics, RNA isolation & purification, RNA metabolism, Gene Expression Regulation, Nerve Tissue Proteins metabolism, Nucleic Acid Hybridization, Spinal Cord chemistry, Spinal Cord metabolism

Abstract

Comparison of cDNA libraries derived from the spinal cord with those derived from the visual cortex by means of forward and reverse subtractive hybridization resulted in the cataloguing of 60 genes differentially expressed in the spinal cord. 1. The differentially expressed genes represent a mixture of novel and known sequences with known and unknown protein products. 2. The possibility that the subtraction process was simply overwhelmed by background sequences was significantly reduced by several observations including comparisons between suppression subtractive hybridization (SSH) and mirror orientation selection (MOS). 3. Nearly half of all genes up-regulated in the spinal cord are of myelin origin. 4. Twenty-five percent of all up-regulated clones in the spinal cord versus the visual cortex are for proteolipid protein. 5. Ten percent of all up-regulated clones in spinal cord versus visual cortex are for ferretin heavy chain, which is known to be produced in oligodendroglial cells in the CNS. 6. Two of the up-regulated sequences, proteolipid protein and N-myc down-regulated gene 4, are identified with genes known to directly affect neuron survival. 7. Two of the up-regulated genes, ferritin and transferrin, are indirectly associated with apoptosis through their ability to sequester iron and reduce free radical formation.

Published

2006