The transient receptor potential channel subfamily V member 1 (TRPV1) functions as the heat and capsaicin receptor. It can be activated by heat, protons, pungent chemicals, and a variety of other endogenous mediators of nociception. TRPV1 is a non-selective cation…
The transient receptor potential channel subfamily V member 1 (TRPV1) functions as the heat and capsaicin receptor. It can be activated by heat, protons, pungent chemicals, and a variety of other endogenous mediators of nociception. TRPV1 is a non-selective cation channel consisting of 6 transmembrane domains (S1-S6), with helices S1-S4 forming the sensing domain and the S5-S6 helices forming the pore domain. Understanding the TRPV1 channel is imperative due to its relation to a variety of human diseases, including cancer, type II diabetes, hyper and hypothermia, and inflammatory disorders of the airways and bladder. Although TRPV1 is the best-studied thermosensitive-TRP channels of all the 28 family members, the molecular underpinning and the contributions of the human TRPV1 pore domain in thermo-sensing remains elusive. Recently, the human TRPV1 sensing domain was found to contribute to heat activation. It was found to undergo a non-denaturing temperature-dependent conformational change. This finding triggered interest in studying the function and the role of the human TRPV1 pore domain in the heat activation process. Specifically, to identify whether heat activation is intrinsic to the pore domain. This thesis paper explores and optimizes the purification protocol of the human TRPV1 pore domain through three different methods. The first method was using a denaturant, the second method was increasing the length of the histidine tags through Q5 insertion, and the third method was incorporating the protein construct into nanodiscs. In addition to the above three methods, size exclusion chromatography and ion-exchange chromatography were utilized after thrombin cleavage to separate the human TRPV1 pore domain from the cleaved MBP deca-histidine tags as well as the impurities.
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Octopus arms employ a complex three dimensional array of musculature, called a muscular hydrostat, which allows for nearly infinite degrees of freedom of movement without the structure of a skeletal system. This study employed Magnetic Resonance Imaging with a Gadoteridol-based contrast agent to…
Octopus arms employ a complex three dimensional array of musculature, called a muscular hydrostat, which allows for nearly infinite degrees of freedom of movement without the structure of a skeletal system. This study employed Magnetic Resonance Imaging with a Gadoteridol-based contrast agent to image the octopus arm and view the internal tissues. Muscle layering was mapped and area was measured using AMIRA image processing and the trends in these layers at the proximal, middle, and distal portions of the arms were analyzed. A total of 39 arms from 6 specimens were scanned to give 112 total imaged sections (38 proximal, 37 middle, 37 distal), from which to ascertain and study the possible differences in musculature. The images revealed significant increases in the internal longitudinal muscle layer percentages between the proximal and middle, proximal and distal, and middle and distal sections of the arms. These structural differences are hypothesized to be used for rapid retraction of the distal segment when encountering predators or noxious stimuli. In contrast, a significant decrease in the transverse muscle layer was found when comparing the same sections. These structural differences are hypothesized to be a result of bending behaviors during retraction. Additionally, the internal longitudinal layer was separately studied orally, toward the sucker, and aborally, away from the sucker. The significant differences in oral and aboral internal longitudinal musculature in proximal, middle, and distal sections is hypothesized to support the pseudo-joint functionality displayed in octopus fetching behaviors. The results indicate that individual octopus arm morphology is more unique than previously thought and supports that internal structural differences exist to support behavioral functionality.
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The entirely soft-tissue anatomy of the octopus arm provides the animal with a large amount of freedom of movement, while still allowing the specimen to support itself despite the lack of a skeletal system. This is made possible through the…
The entirely soft-tissue anatomy of the octopus arm provides the animal with a large amount of freedom of movement, while still allowing the specimen to support itself despite the lack of a skeletal system. This is made possible through the use of various muscle layers within the octopus arm, which act as muscular hydrostats. Magnetic Resonance imaging of the octopus arm was employed to view the muscle layers within the octopus arm and observe trends and differences in these layers at the proximal, middle, and distal portions of the arms. A total of 39 arms from 6 specimens were imaged to give 112 total imaged sections (38 proximal, 37 middle, 37 distal). Significant increases in both the internal longitudinal muscle layer and the nervous core were found between the proximal and middle, proximal and distal, and middle and distal sections of the arms. This could reflect selection for these structures distally in the octopus arm for predator or other noxious stimuli avoidance. A significant decrease in the transverse muscle layer was found in the middle and distal sections of the arms. This could reflect selection for elongation in the proximal portion of the octopus arm or could be the result of selection for the internal longitudinal muscle layer and nervous core distally. Previous studies on Octopus vulgaris showed a preference for using the proximal arms in the pushing movement of crawling and a preference for using the anterior arms in exploring behaviors (Levy et al., 2015 and Byrne et al., 2006). Differences between the anterior and posterior arms for the transverse muscle layer, internal longitudinal muscle layer, and the nervous core were insignificant, reflecting a lack of structure-function relationships. This could also be due to a low sample size. Differences between the left and right arms for the transverse muscle layer, internal longitudinal muscle layer, and the nervous core were insignificant, supporting previous evidence that left versus right eye and arm preferences in octopus are not population-wide, but individual. Some slight trends can be found for individual arms, but the sample size was too small to make definitive statements regarding differences among specific arms.
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Solid-state NMR and molecular dynamics (MD) simulations are presented to help elucidate the molecular secondary structure of poly(Gly-Gly-X), which is one of the most common structural repetitive motifs found in orb-weaving dragline spider silk proteins. The combination of NMR and…
Solid-state NMR and molecular dynamics (MD) simulations are presented to help elucidate the molecular secondary structure of poly(Gly-Gly-X), which is one of the most common structural repetitive motifs found in orb-weaving dragline spider silk proteins. The combination of NMR and computational experiments provides insight into the molecular secondary structure of poly(Gly-Gly-X) segments and provides further support that these regions are disordered and primarily non-β-sheet. Furthermore, the combination of NMR and MD simulations illustrate the possibility for several secondary structural elements in the poly(Gly-Gly-X) regions of dragline silks, including β-turns, 310-helicies, and coil structures with a negligible population of α-helix observed.
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Solving high-resolution structures for membrane proteins continues to be a daunting challenge in the structural biology community. In this study we report our high-resolution NMR results for a transmembrane protein, outer envelope protein of molar mass 16 kDa (OEP16), an…
Solving high-resolution structures for membrane proteins continues to be a daunting challenge in the structural biology community. In this study we report our high-resolution NMR results for a transmembrane protein, outer envelope protein of molar mass 16 kDa (OEP16), an amino acid transporter from the outer membrane of chloroplasts. Three-dimensional, high-resolution NMR experiments on the [superscript 13]C, [superscript 15]N, [superscript 2]H-triply-labeled protein were used to assign protein backbone resonances and to obtain secondary structure information. The results yield over 95% assignment of N, H[subscript N], CO, C[subscript α], and C[subscript β] chemical shifts, which is essential for obtaining a high resolution structure from NMR data. Chemical shift analysis from the assignment data reveals experimental evidence for the first time on the location of the secondary structure elements on a per residue basis. In addition T[subscript 1Z] and T[subscript 2] relaxation experiments were performed in order to better understand the protein dynamics. Arginine titration experiments yield an insight into the amino acid residues responsible for protein transporter function. The results provide the necessary basis for high-resolution structural determination of this important plant membrane protein.
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