Solutions to Genetics Day 6 Interpretation Questions

... one thing that could have prevented this from occurring. We used a modified λ phage that carried the mini-TN10 transposon to deliver the DNA to the bacterial cell. This phage was no longer lytic or lysogenic and the INT sites of the phage DNA were removed to prevent specific insertions. The gene enc ...

Document

... cleaves on the carboxyl side of basic side chains (Lys, Arg), whereas chymotrypsin cleaves on the carboxyl side of aromatics (Phe, Tyr, Trp) The active site consists of a “catalytic triad”: 1) Serine, to which the substrate binds 2) Histidine, which has the ability to donate and accept protons. 3) A ...

Myriad myPath® Melanoma Technical Specifications

... This gene expression signature is intended for the in vitro analysis of melanocytic neoplasms to aid in the diagnosis of the lesion as benign or malignant. This is an adjunctive assay and should be used in conjunction with clinical data and histopathological features. Summary and Explanation Melanom ...

PcrA Helicase Tightly Couples ATP Hydrolysis to Unwinding Double

... rapid mixing of RepD with Junction 3, in which the fluorescein is attached at the 50 -end of the ICRII arm rather than the end of the duplex. The traces (Figure 4a) show a rapid rise in anisotropy followed by a slow decrease to a level below that of the initial DNA. This would be expected from rapid ...

18–2 Modern Evolutionary Classification

... role in cellular respiration, was chosen for study because it is present in most organisms. Point out how closely the phylogenetic tree based on this single important protein resembles traditional phylogenetic trees based on other kinds of evidence. ...

Small-Subunit Ribosomal RNA Sequence from

... determined (Sogin et al. 1986). It must also be remembered that only a single, cloned copy of the approximately 4,000 genes per cell was sequenced and that variation between genes may exist, although we have no evidence for this. The unique structure of the Naegleria rDNA can be reassessed in light ...

Metagenomics: DNA sequencing of environmental samples

... Natural samples contain DNA in a variety of packages, including free DNA, virus particles, and prokaryotic and eukaryotic cells. These can be suspended in water, bound to a solid matrix like soil, or encased in a biofilm or tissue. Extraction methods must be chosen carefully based on the medium and ...

a 2-sided "mini-poster" version. - Southeast Missouri State University

... strips, and a profile of resistance to 17 antibiotics was determined using the Kirby-Bauer agar diffusion test. Chromosomal DNA was extracted by phenol:chloroform separation in the presence of CTAB detergent and by DNeasy. Plasmid extractions were performed with the Qiagen mini-prep kit and the Wi ...

mRNA over-expression/rescue

... 3. Mutant (today) or morpholino (tomorrow) rescue 4. Epistasis: what genes can and cannot rescue your mutant? Where does your mutant gene lie in a pathway? Why inject DNA? • Gain-of-function experiments: over & ectopic expression • Dominant negative expts • Promoter analysis • Transgenics--in vivo l ...

PPT presentation

... • Amino acid pairs are classified into two types: identical and non-identical • Non-identical pairs are scored 0 and identical pairs given a positive score (usually 1) • The scoring scheme is generally considered less effective than schemes that weight non-identical pairs ...

BIOTECHNOLOGY B.Sc. Semester III

... a. Mechanism of enzyme catalysis- Acid base catalysis, covalent catalysis, metal ion catalysis b. Enzyme kinetics- Michaelis-Menten equation, Lineweaver- Burke plot c. Enzyme inhibition- Reversible inhibition, irreversible inhibition, d. Factors affecting enzyme activity- concentration of enzyme, co ...

Basic quantitative genetics, the “breeders equation

... Clearly the response to selection will be usually be less than the selection differential: R < S. Darwin recognized this, which is part of his reasoning for suggesting blending inheritance. h2 is simply the scaling factor that gives us the response to selection as a proportion of the selection diffe ...

3.1 Review PBS

...  DNA is too large and fragile to leave the nucleus. ...

condensed version - FSU Biology

... OK, given your own experimentally derived nucleotide or amino acid sequence, or one that you’ve found in a database, what more can we learn about its biological function? ...

Physiology is rocking the foundations of evolutionary biology

... Third, following genetic change, natural selection leads to particular gene variants (alleles) increasing in frequency within the population. Those variants are said to confer an advantage in terms of fitness on the individuals concerned, which therefore increasingly dominate the population. By this ...

Enzymes - africangreyparrott.com

Enzymes

Terminal Transferase Reaction Buffer Pack | New England Biolabs

... Quality Control Assays The following Quality Control Tests are performed on each new lot and meet the specifications designated for the product. Individual lot data can be found on the Product Summary Sheet/Datacard or Manual which can be found in the Supporting Documents section of this page. Furth ...

Answers to Mastering Concepts Questions

... 1. How do acids and bases affect a solution’s H+ concentration? An acid adds H+ to the solution, whereas a base absorbs H+. 2. How do the values of 0, 7, and 14 relate to the pH scale? 0 and 14 on the pH scale represent the strongest acidic and basic solutions respectively, while 7 is the value of a ...

Working With Enzymes - Southern Biological

... breakdown of starch – but they can be significantly different biochemicals. Most commercial enzymes these days are derived from bacterial or fungal cultures that can be grown in large bioreactors to maximize the yield. Rather than purifying the product to a high degree, commercial enzymes are usuall ...

Introduction

... GR Safe I is a new, safe nucleic acid stain for detecting double-stranded DNA, single-stranded DNA, and RNA in agarose gel. It can be used for replacing mutagenic ethidium bromide (EB). GR Safe emits green fluorescence when bound to dsDNA and red fluorescence when bound to ssDNA or RNA. This new sta ...

Biomarkers – Alessandra Ferlini

... Peter Bram ‘t Hoen Elizabeth McNally ...

Photosynthesis

... Transcription activators bind to regions of DNA called enhancers. Might be brought near region of promoter by hairpin loops in DNA. Always present in cell, but most likely have to be activated before they will bind to DNA ...

Enzyme Activity

... Inhibitors are chemicals that reduce the rate of enzymic reactions. The are usually specific and they work at low concentrations. They block the enzyme but they do not usually destroy it. ...

Properties of Enzymes

... Properties of Enzymes ...

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Deoxyribozyme

Deoxyribozymes, also called DNA enzymes, DNAzymes, or catalytic DNA, are DNA oligonucleotides that are capable of catalyzing specific chemical reactions, similar to the action of other biological enzymes, such as proteins or ribozymes (enzymes composed of RNA).However, in contrast to the abundance of protein enzymes in biological systems and the discovery of biological ribozymes in the 1980s,there are no known naturally occurring deoxyribozymes.Deoxyribozymes should not be confused with DNA aptamers which are oligonucleotides that selectively bind a target ligand, but do not catalyze a subsequent chemical reaction.With the exception of ribozymes, nucleic acid molecules within cells primarily serve as storage of genetic information due to its ability to form complementary base pairs, which allows for high-fidelity copying and transfer of genetic information. In contrast, nucleic acid molecules are more limited in their catalytic ability, in comparison to protein enzymes, to just three types of interactions: hydrogen bonding, pi stacking, and metal-ion coordination. This is due to the limited number of functional groups of the nucleic acid monomers: while proteins are built from up to twenty different amino acids with various functional groups, nucleic acids are built from just four chemically similar nucleobases. In addition, DNA lacks the 2'-hydroxyl group found in RNA which limits the catalytic competency of deoxyribozymes even in comparison to ribozymes.In addition to the inherent inferiority of DNA catalytic activity, the apparent lack of naturally occurring deoxyribozymes may also be due to the primarily double-stranded conformation of DNA in biological systems which would limit its physical flexibility and ability to form tertiary structures, and so would drastically limit the ability of double-stranded DNA to act as a catalyst; though there are a few known instances of biological single-stranded DNA such as multicopy single-stranded DNA (msDNA), certain viral genomes, and the replication fork formed during DNA replication. Further structural differences between DNA and RNA may also play a role in the lack of biological deoxyribozymes, such as the additional methyl group of the DNA base thymidine compared to the RNA base uracil or the tendency of DNA to adopt the B-form helix while RNA tends to adopt the A-form helix. However, it has also been shown that DNA can form structures that RNA cannot, which suggests that, though there are differences in structures that each can form, neither is inherently more or less catalytic due to their possible structural motifs.

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Deoxyribozyme