1 / 92

Chapter 6

Chapter 6. A Tour of the Cell. Overview: The Importance of Cells All organisms are made of cells The cell is the simplest collection of matter that can live. 10 µm . Cell structure is correlated to cellular function. Figure 6.1.

kera
Télécharger la présentation

Chapter 6

An Image/Link below is provided (as is) to download presentation Download Policy: Content on the Website is provided to you AS IS for your information and personal use and may not be sold / licensed / shared on other websites without getting consent from its author. Content is provided to you AS IS for your information and personal use only. Download presentation by click this link. While downloading, if for some reason you are not able to download a presentation, the publisher may have deleted the file from their server. During download, if you can't get a presentation, the file might be deleted by the publisher.

E N D

Presentation Transcript

  1. Chapter 6 A Tour of the Cell

  2. Overview: The Importance of Cells • All organisms are made of cells • The cell is the simplest collection of matter that can live

  3. 10 µm • Cell structure is correlated to cellular function Figure 6.1

  4. Concept 6.1: To study cells, biologists use microscopes and the tools of biochemistry

  5. Microscopy • Scientists use microscopes to visualize cells too small to see with the naked eye

  6. Light microscopes (LMs) • Pass visible light through a specimen • Magnify cellular structures with lenses

  7. 10 m Human height 1 m Length of some nerve and muscle cells 0.1 m Light microscope Chicken egg 1 cm Frog egg 1 mm 100 µm Most plant and Animal cells Electron microscope 10 µ m NucleusMost bacteriaMitochondrion 1 µ m Electron microscope Smallest bacteria 100 nm Viruses 10 nm Ribosomes Proteins Lipids 1 nm Small molecules Figure 6.2 Atoms 0.1 nm • Different types of microscopes • Can be used to visualize different sized cellular structures Unaided eye Measurements 1 centimeter (cm) = 102 meter (m) = 0.4 inch 1 millimeter (mm) = 10–3 m 1 micrometer (µm) = 10–3 mm = 10–6 m 1 nanometer (nm) = 10–3 mm = 10–9 m

  8. RESULT TECHNIQUE (a) Brightfield (unstained specimen). Passes light directly through specimen. Unless cell is naturally pigmented or artificially stained, image has little contrast. [Parts (a)–(d) show a human cheek epithelial cell.] 50 µm (b) Brightfield (stained specimen).Staining with various dyes enhances contrast, but most staining procedures require that cells be fixed (preserved). (c) Phase-contrast. Enhances contrast in unstained cells by amplifying variations in density within specimen; especially useful for examining living, unpigmented cells. Figure 6.3 • Use different methods for enhancing visualization of cellular structures

  9. (d) (e) Fluorescence. Shows the locations of specific molecules in the cell by tagging the molecules with fluorescent dyes or antibodies. These fluorescent substances absorb ultraviolet radiation and emit visible light, as shown here in a cell from an artery. 50 µm (f) Confocal. Uses lasers and special optics for “optical sectioning” of fluorescently-stained specimens. Only a single plane of focus is illuminated; out-of-focus fluorescence above and below the plane is subtracted by a computer. A sharp image results, as seen in stained nervous tissue (top), where nerve cells are green, support cells are red, and regions of overlap are yellow. A standard fluorescence micrograph (bottom) of this relatively thick tissue is blurry. 50 µm Differential-interference-contrast (Nomarski). Like phase-contrast microscopy, it uses optical modifications to exaggerate differences in density, making the image appear almost 3D.

  10. Electron microscopes (EMs) • Focus a beam of electrons through a specimen (TEM) or onto its surface (SEM)

  11. TECHNIQUE RESULTS 1 µm Cilia (a) Scanning electron micro- scopy (SEM). Micrographs taken with a scanning electron micro- scope show a 3D image of the surface of a specimen. This SEM shows the surface of a cell from a rabbit trachea (windpipe) covered with motile organelles called cilia. Beating of the cilia helps move inhaled debris upward toward the throat. • The scanning electron microscope (SEM) • Provides for detailed study of the surface of a specimen Figure 6.4 (a)

  12. Longitudinal section of cilium Cross section of cilium 1 µm (b) Transmission electron micro- scopy (TEM). A transmission electron microscope profiles a thin section of a specimen. Here we see a section through a tracheal cell, revealing its ultrastructure. In preparing the TEM, some cilia were cut along their lengths, creating longitudinal sections, while other cilia were cut straight across, creating cross sections. • The transmission electron microscope (TEM) • Provides for detailed study of the internal ultrastructure of cells Figure 6.4 (b)

  13. Isolating Organelles by Cell Fractionation • Cell fractionation • Takes cells apart and separates the major organelles from one another

  14. The centrifuge • Is used to fractionate cells into their component parts

  15. APPLICATION TECHNIQUE • The process of cell fractionation Cell fractionation is used to isolate (fractionate) cell components, based on size and density. First, cells are homogenized in a blender to break them up. The resulting mixture (cell homogenate) is then centrifuged at various speeds and durations to fractionate the cell components, forming a series of pellets. Figure 6.5

  16. Homogenization Tissue cells 1000 g (1000 times the force of gravity) 10 min Homogenate Differential centrifugation Supernatant poured into next tube 20,000 g 20 min 80,000 g 60 min Pellet rich in nuclei and cellular debris 150,000 g 3 hr Pellet rich in mitochondria (and chloro- plasts if cells are from a plant) Pellet rich in “microsomes” (pieces of plasma mem- branes and cells’ internal membranes) Pellet rich in ribosomes Figure 6.5

  17. RESULTS In the original experiments, the researchers used microscopy to identify the organelles in each pellet, establishing a baseline for further experiments. In the next series of experiments, researchers used biochemical methods to determine the metabolic functions associated with each type of organelle. Researchers currently use cell fractionation to isolate particular organelles in order to study further details of their function. Figure 6.5

  18. Concept 6.2: Eukaryotic cells have internal membranes that compartmentalize their functions • Two types of cells make up every organism • Prokaryotic • Eukaryotic

  19. Comparing Prokaryotic and Eukaryotic Cells • All cells have several basic features in common • They are bounded by a plasma membrane

  20. They contain a semifluid substance called the cytosol • They contain chromosomes • They all have ribosomes

  21. Prokaryotic cells • Do not contain a nucleus • Have their DNA located in a region called the nucleoid

  22. Pili: attachment structures on the surface of some prokaryotes Nucleoid: region where the cell’s DNA is located (not enclosed by a membrane) Ribosomes: organelles that synthesize proteins Plasma membrane: membrane enclosing the cytoplasm Cell wall: rigid structure outside the plasma membrane Capsule: jelly-like outer coating of many prokaryotes Bacterialchromosome 0.5 µm Flagella: locomotion organelles of some bacteria (a) A typical rod-shaped bacterium (b) A thin section through the bacterium Bacillus coagulans (TEM) Figure 6.6 A, B

  23. Eukaryotic cells • Contain a true nucleus, bounded by a membranous nuclear envelope • Are generally quite a bit bigger than prokaryotic cells

  24. The logistics of carrying out cellular metabolism sets limits on the size of cells

  25. Surface area increases while total volume remains constant 5 1 1 Total surface area (height  width  number of sides  number of boxes) 6 150 750 Total volume (height  width  length  number of boxes) 125 125 1 Surface-to-volume ratio (surface area  volume) 6 12 6 • A smaller cell • Has a higher surface to volume ratio, which facilitates the exchange of materials into and out of the cell Figure 6.7

  26. Outside of cell Hydrophilic region TEM of a plasma membrane. The plasma membrane, here in a red blood cell, appears as a pair of dark bands separated by a light band. (a) Inside of cell 0.1 µm Hydrophobic region Hydrophilic region Phospholipid Proteins (b) Structure of the plasma membrane • The plasma membrane • Functions as a selective barrier • Allows sufficient passage of nutrients and waste Carbohydrate side chain Figure 6.8 A, B

  27. A Panoramic View of the Eukaryotic Cell • Eukaryotic cells • Have extensive and elaborately arranged internal membranes, which form organelles

  28. Plant and animal cells • Have most of the same organelles

  29. Nuclear envelope ENDOPLASMIC RETICULUM (ER) NUCLEUS Nucleolus Rough ER Smooth ER Chromatin Flagelium Plasma membrane Centrosome CYTOSKELETON Microfilaments Intermediate filaments Ribosomes Microtubules Microvilli Golgi apparatus Peroxisome In animal cells but not plant cells: Lysosomes Centrioles Flagella (in some plant sperm) Lysosome Mitochondrion • A animal cell Figure 6.9

  30. Nuclear envelope Rough endoplasmic reticulum Nucleolus NUCLEUS Chromatin Smooth endoplasmic reticulum Centrosome Ribosomes (small brwon dots) Central vacuole Tonoplast Golgi apparatus Microfilaments Intermediate filaments Microtubules Mitochondrion Peroxisome Plasma membrane Chloroplast Cell wall Plasmodesmata Wall of adjacent cell • A plant cell CYTOSKELETON In plant cells but not animal cells: Chloroplasts Central vacuole and tonoplast Cell wall Plasmodesmata Figure 6.9

  31. Concept 6.3: The eukaryotic cell’s genetic instructions are housed in the nucleus and carried out by the ribosomes

  32. The Nucleus: Genetic Library of the Cell • The nucleus • Contains most of the genes in the eukaryotic cell

  33. Nucleus Nucleus 1 µm Nucleolus Chromatin Nuclear envelope: Inner membrane Outer membrane Nuclear pore Pore complex Rough ER Surface of nuclear envelope. 1 µm Ribosome 0.25 µm Close-up of nuclear envelope Nuclear lamina (TEM). Pore complexes (TEM). • The nuclear envelope • Encloses the nucleus, separating its contents from the cytoplasm Figure 6.10

  34. Ribosomes: Protein Factories in the Cell • Ribosomes • Are particles made of ribosomal RNA and protein

  35. Ribosomes Cytosol Free ribosomes Bound ribosomes Large subunit Small subunit 0.5 µm TEM showing ER and ribosomes Diagram of a ribosome • Carry out protein synthesis ER Endoplasmic reticulum (ER) Figure 6.11

  36. Concept 6.4: The endomembrane system regulates protein traffic and performs metabolic functions in the cell • The endomembrane system • Includes many different structures

  37. The Endoplasmic Reticulum: Biosynthetic Factory • The endoplasmic reticulum (ER) • Accounts for more than half the total membrane in many eukaryotic cells

  38. Smooth ER Nuclear envelope Rough ER ER lumen Cisternae Ribosomes Transitional ER Transport vesicle 200 µm Smooth ER Rough ER • The ER membrane • Is continuous with the nuclear envelope Figure 6.12

  39. There are two distinct regions of ER • Smooth ER, which lacks ribosomes • Rough ER, which contains ribosomes

  40. Functions of Smooth ER • The smooth ER • Synthesizes lipids • Metabolizes carbohydrates • Stores calcium • Detoxifies poison

  41. Functions of Rough ER • The rough ER • Has bound ribosomes • Produces proteins and membranes, which are distributed by transport vesicles

  42. The Golgi Apparatus: Shipping and Receiving Center • The Golgi apparatus • Receives many of the transport vesicles produced in the rough ER • Consists of flattened membranous sacs called cisternae

  43. Functions of the Golgi apparatus include • Modification of the products of the rough ER • Manufacture of certain macromolecules

  44. cis face (“receiving” side of Golgi apparatus) 5 3 4 6 2 1 Vesicles coalesce to form new cis Golgi cisternae Vesicles move from ER to Golgi 0.1 0 µm Vesicles also transport certain proteins back to ER Cisternae Cisternal maturation: Golgi cisternae move in a cis- to-trans direction Vesicles form and leave Golgi, carrying specific proteins to other locations or to the plasma mem- brane for secretion trans face (“shipping” side of Golgi apparatus) Vesicles transport specific proteins backward to newer Golgi cisternae • Functions of the Golgi apparatus Golgi apparatus Figure 6.13 TEM of Golgi apparatus

  45. Lysosomes: Digestive Compartments • A lysosome • Is a membranous sac of hydrolytic enzymes • Can digest all kinds of macromolecules

  46. 1 µm Nucleus Lysosome Hydrolytic enzymes digest food particles Food vacuole fuses with lysosome Lysosome contains active hydrolytic enzymes Digestive enzymes Lysosome Plasma membrane Digestion Food vacuole (a) Phagocytosis: lysosome digesting food • Lysosomes carry out intracellular digestion by • Phagocytosis Figure 6.14 A

  47. Lysosome containing two damaged organelles 1 µ m Mitochondrion fragment Peroxisome fragment Lysosome fuses with vesicle containing damaged organelle Hydrolytic enzymes digest organelle components Lysosome Digestion Vesicle containing damaged mitochondrion (b) Autophagy: lysosome breaking down damaged organelle • Autophagy Figure 6.14 B

  48. Vacuoles: Diverse Maintenance Compartments • A plant or fungal cell • May have one or several vacuoles

  49. Food vacuoles • Are formed by phagocytosis • Contractile vacuoles • Pump excess water out of protist cells

  50. Central vacuole Cytosol Tonoplast Nucleus Central vacuole Cell wall Chloroplast 5 µm • Central vacuoles • Are found in plant cells • Hold reserves of important organic compounds and water Figure 6.15

More Related