beta-Sheet forming peptides by design| Control of folding and applications

Takor, Gaius A.

10 May 2016

<p> The focus of the present research is the synthesis of polypeptides for the study of protein folding and misfolding and for the development of novel polypeptide-based optical antennas in nanotechnology. It is hypothesized that simple polypeptides can be used as models to mimic <i>in vivo</i> folding of globular proteins. Desired repetitive polypeptides were genetically encoded and expressed in <i>E. coli</i> using conventional methods and characterized using a variety of spectroscopic (including circular dichroism (CD), deep UV resonance Raman (DUVRR), UV-vis and fluorescence) and microscopic (atomic force microscopy (AFM) and transmission electron microscopy (TEM)) techniques. The polypeptides predominantly formed bilayer, fibrillar structures with a cross &beta;-core. <b>YEHK21-YE8</b>, a chimeric polypeptide, folded within three days. The folding/fibrillation of the chimeric construct illuminates the controlling factors and hence suggests the importance of those factors in amyloidogenic diseases. <b>YE8</b> and <b>YE8</b> derivatives illustrated the role of proline in &beta;-sheet formation. The EW polypeptide models elucidated the influence of tryptophan residues and the degree of polymerization on folding. The study of <b>EW14C1</b> and <b>EW21C1</b> demonstrated light-harvesting properties when labeled with a suitable dye.</p>

Molecular biology|Genetics|Biochemistry

A Mutational-Functional Analysis of the Escherichia coli Macrodomain Protein, YmdB

Smith, Alexandra Kimberly

29 January 2019

<p> Gene expression pathways exhibit many "twists and turns," with theoretically numerous ways in which the pathways can be regulated by both negative and positive feedback mechanisms. A key step in gene expression is RNA maturation (RNA processing), which in the bacterial cell can be accomplished through RNA binding and enzymatic cleavages. The well-characterized bacterial protein Ribonuclease III (RNase III), is a conserved, double-stranded(ds)-specific ribonuclease. In the gram-negative bacterium <i>Escherichia coli</i>, RNase III catalytic activity is subject to both positive and negative regulation. A recent study has indicated that an <i>E. coli</i> protein, YmdB, may negatively regulate RNase III catalytic activity. It has been proposed that YmdB inhibition of RNase III may be part of an adaptive, post-transcriptional physiological response to cellular stress. </p><p> In <i>E. coli</i>, the model organism in this study, YmdB protein is encoded by the single <i>ymdB</i> gene, and has a predicted molecular mass of &sim;18.8 kDa. YmdB has been classified as a macrodomain protein, as it exhibits a characteristic fold that specifically provides an ADP-ribose (ADPR) binding site. While YmdB can bind ADPR with good affinity, there may be additional ligands for the binding site. Thus, YmdB protein may interact with other components in the cell, which in turn could modulate the interaction of YmdB with RNase III. </p><p> In previous research conducted within the Nicholson laboratory at Temple University, affinity-purified <i>Escherchia coli(Ec)</i> YmdB and <i> Aquifex aeolicus (Aa)</i> YmdB were found to exhibit ribonucleolytic activity. This observation initiated the long-term goal of learning how YmdB regulates RNase III, and how the ribonucleolytic activity of YmdB may be involved in this process. The specific goal of this thesis project was to further characterize the ribonucleolytic activity of <i>Ec-</i>YmdB through site-specific mutational analysis. Mutations were introduced into a proposed adenine-binding pocket previously identified by crystallography and by molecular modeling. The adenine-binding pocket is a region within the macrodomain fold where ADP-ribose could bind. The mutations were examined for their effect on <i>Ec-</i>YmdB cleavage of a model RNA, R1.1. The results of this study will contribute to the development of a model describing how the ribonucleolytic activity of YmdB is regulated.</p><p>