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Proteins
Biochemistry and Biotechnology
Gary Walsh
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Proteins
Biochemistry and Biotechnology
Gary Walsh
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About This Book
Proteins Biochemistry and Biotechnology 2e is a definitive source of information for all those interested in protein science, and particularly the commercial production and isolation of specific proteins, and their subsequent utilization for applied purposes in industry and medicine. Fully updated throughout with new or fundamentally revised sections on proteomics as, bioinformatics, protein glycosylation and engineering, well as sections detailing advances in upstream processing and newer protein applications such as enzyme-based biofuel production this new edition has an increased focus on biochemistry to ensure the balance between biochemisty and biotechnology, enhanced with numerous case studies. This second edition is an invaluable text for undergraduates of biochemistry and biotechnology but will also be relevant to students of microbiology, molecular biology, bioinformatics and any branch of the biomedical sciences who require a broad overview of the various medical, diagnostic and industrial uses of proteins. ā¢ Provides a comprehensive overview of all aspects of protein biochemisty and protein biotechnology
ā¢ Includes numerous case studies
ā¢ Increased focus on protein biochemistry to ensure balance between biochemisty and biotechnology
ā¢ Includes new section focusing on proteomics as well as sections detailing protein function and enzyme-based biofuel production "With the potential of a standard reference source on the topic, any molecular biotechnologist will profit greatly from having this excellent book. " ( Engineering in Life Sciences, 2004; Vol 5; No. 5) "Few texts would be considered competitors, and none compare favorably." ( Biochemistry and Molecular Education, July/August 2002) "...The book is well written, making it informative and easy to read..." ( The Biochemist, June 2002)
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Chapter 1
Proteins and proteomics
Throughout this book, I will consider various aspects of protein structure, function, engineering and application. Traditionally, protein science focused on isolating and studying one protein at a time. However, since the 1990s, advances in molecular biology, analytical technologies and computing has facilitated the study of many proteins simultaneously, which has led to an information explosion in this area. In this chapter such proteomic and related approaches are reviewed.
1.1 Proteins, an introduction
While we consider protein structure in detail in Chapter 2, for the purposes of this chapter it is necessary to provide a brief overview of the topic. Proteins are macromolecules consisting of one or more polypeptide chains (Table 1.1). Each polypeptide consists of a chain of amino acids linked together by peptide (amide) bonds. The exact amino acid sequence is determined by the gene coding for that specific polypeptide. When synthesized, a polypeptide chain folds up, assuming a specific three-dimensional shape (i.e. a specific conformation) that is unique to the protein. The conformation adopted depends on the polypeptideās amino acid sequence, and this conformation is largely stabilized by multiple, weak interactions. Overall, a proteinās structure can described at up to four different levels.
- Primary structure: the specific amino acid sequence of its polypeptide chain(s), along with the exact positioning of any disulfide bonds present.
- Secondary structure: regular recurring arrangements of adjacent amino acid residues, often over relatively short contiguous sequences within the protein backbone. The common secondary structures are the Ī±-helix and Ī²-strands.
- Tertiary structure: the three-dimensional arrangement of all the atoms which contribute to the polypeptide. In other words, the overall three-dimensional structure (conformation) of a polypeptide chain, which usually contains several stretches of secondary structure interrupted by less ordered regions such as bends/loops.
- Quaternary structure: the overall spatial arrangement of polypeptide subunits within a protein composed of two or more polypeptides.
The majority of proteins derived from eukaryotes undergo covalent modification either during, or more commonly after, their ribosomal synthesis. This gives rise to the concept of co-translational and post-translational modifications, although both modifications are often referred to simply as post-translational modifications (PTMs), and such modifications can influence protein structure and/or function. Proteins are also sometimes classified as āsimpleā or āconjugatedā. Simple proteins consist exclusively of polypeptide chain(s) with no additional chemical components being present or being required for biological activity. Conjugated proteins, in addition to their polypeptide components, contain one or more non-polypeptide constituents known as prosthetic groups. The most common prosthetic groups found in association with proteins include carbohydrates (glycoproteins), phosphate groups (phosphoproteins), vitamin derivatives (e.g. flavoproteins) and metal ions (metalloproteins).
Table 1.1 Selected examples of proteins. The number of polypeptide chains and amino acid residues constituting the protein are listed, along with its molecular mass and biological function.
| Protein | Polypeptide chains | Total no. of amino acids | Molecular mass (Da) | Biological function |
| Insulin (human) | 2 | 51 | 5800 | Complex, but includes regulation of blood glucose levels |
| Lysozyme (egg) | 1 | 129 | 13,900 | Enzyme capable of degrading peptidoglycan in bacterial cell walls |
| Interleukin-2 (human) | 1 | 133 | 15,400 | T-lymphocyte-derived polypeptide that regulates many aspects of immunity |
| Erythropoietin (human) | 1 | 165 | 36,000 | Hormone which stimulates red blood cell production |
| Chymotrypsin (bovine) | 3 | 241 | 21,600 | Digestive proteolytic enzyme |
| Subtilisin (Bacillus amyloliquefaciens) | 1 | 274 | 27,500 | Bacterial proteolytic enzyme |
| Tumour necrosis factor (human TNF-Ī±) | 3 | 471 | 52,000 | Mediator of inflammation and immunity |
| Haemoglobin (human) | 4 | 574 | 64,500 | Gas transport |
| Hexokinase (yeast) | 2 | 800 | 102,000 | Enzyme capable of phosphorylating selected monosaccharides |
| Glutamate dehydrogenase (bovine) | ~40 | ~8300 | ~1,000,000 | Enzyme that interconverts glutamate and Ī±-ketoglutarate and NH4+ |
1.2 Genes, genomics and proteomics
The term āgenomeā refers to the entire complement of hereditary information present in an organism or virus. In the overwhelming majority of cases it is encoded in DNA, although some viruses use RNA as their genetic material. The term āgenomicsā refers to the systematic study of the entire genome of an organism. Its core aims are to:
- sequence the entire DNA complement of the cell; and
- to physically map the genome arrangement (assign exact positions in the genome to the various genes and non-coding regions).
Prior to the 1990s, the sequencing and study of a single gene represented a significant task. However, improvements in sequencing technologies and the development of more highly automated hardware systems now renders DNA sequencing considerably faster, cheaper and more accurate. Cutting-edge sequencing systems now in development are claimed capable of sequencing small genomes in minutes, and a full human genome sequence in a matter of hours and for a cost of approximately $1000. By early 2014, the genomes online database (GOLD; www.genomesonline.org), which monitors genome studies worldwide, documented some 36,000 ongoing/complete genome projects, and the rate of completion of such studies is growing exponentially. From the perspective of protein science, the most significant consequence of genome data is that it provides full sequence information pertinent to every protein the organism can produce.
The term āproteomeā refers to the entire complement of proteins expressed by a specific cell/organism. It is more complex than the corresponding genome in that:
- at any given time a proportion of genes are not being expressed;
- of those genes that are expressed, some are expressed at higher levels than others;
- the proteome is dynamic rather than static because the exact subset of proteins expressed (and the level at which they are expressed) in any cell changes with time in response to a myriad of environmental and genetic influences;
- for eukaryotes, a single gene can effectively encode more than one polypeptide if its mRNA undergoes differential splicing (Figure 1.1);
- many eukaryotic proteins undergo PTM.
The last two points in particular generally sigify that the number of proteins comprising a eukaryotic organismās proteome can far exceed the number of genes present in its genome. For example, the human genome comprises approximately 22,000 genes whereas the number of distinct protein structures present may exceed 1 million, with any one cell containing an estimated average of approximately 10,000 proteins.
Figure 1.1 Differential splicing of mRNA can yield different polypeptide products. Transcription of a gene sequence yields a āprimary transcriptā RNA. This contains coding regions (exons) and non-coding regions (introns). A major feature of the subsequent processing of the primary transcript is āsplicingā, the process by which introns...