Chapter-7-Microbial-Growth-and-Growth-control-微生物学-教学课件-英文版.ppt
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- Chapter Microbial Growth and control 微生物学 教学 课件 英文
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1、Chapter 7 Microbial Growth and Growth control7.1 Overview of Cell Growth7.2 Population Growth 7.3 Measurement of Growth7.4 Continuous Culture:The Chemostat 7.5 Effect of Environment on Growth7.6 Growth Control 7.7 Viral Control7.8 Fungal Control Chapter outline Concepts Microbial growth is defined a
2、s an increase in cellular constituents and may result in an increase in a microorganisms size,population number,or both.A wide variety of techniques can be used to study microbial growth by following changes in the total cell number,the population of viable microorganisms,or the cell mass.Solid obje
3、cts can be sterilized by physical agents such as heat and radiation;Liquids and gases are sterilized by heat,radiation,and filtration through the proper filter.A knowledge of methods used for microbial control is essential for personal and public safety.G1 Primary growth phase of the cell during whi
4、ch cell enlargement occurs,a gap phase separating cell growth from replication of the genomeS Phase in which replication of the genome occursG2 Phase in which the cell prepares for separation of the replicated genomes,this phase includes synthesis of microtubules and condensation of DNA to form cohe
5、rent chromosomes,a gap phase separating chromosome replication from miosis.M Phase called miosis during which the microtubular apparatus is associated and subsequently used to pull apart the sister chromosomes.Cell life cycle in Eukaryotic cellsEukaryotic cell:Prokaryotic cell:G1 S G2 M G1 R DMost b
6、acterial cells reproduce asexually by binary fision,a process in which a cell divides to produce two nearly equal-sized progeny cells.Three processes:Increase in cell size(cell elongation)DNA replication Cell divisionBinary fisionT125.gif7.2 Population GrowthGrowth is defined as an increase in the n
7、umber of microbial cells in a population.Growth rate is the change in cell number or cell mass per unit time.The interval for the formation of two cells from one is called a generation.The time required for this to occur is called the generation time.A growth experiment beginning with a single cell
8、having a doubling time of 30 min is presented.This pattern of population increase,where the number of cells doubles during each unit time period,is referred to as exponential growth.Exponential Growth N=N02n N=final cell number.N0=initial cell number,and n=number of generations.n=(log N0 log N)/log
9、2 =(log N0 log N)/0.301=3.3(log N log N0).The generation time g of the cell population is calculated as t/n,where t is simply the hours or minutes of exponential growth.Calculating Generation TimesGrowth Cycle of PopulationsA typical growth curve for a population of cells can be divided into several
10、 distinct phases called the lag phase,exponential phase,stationary phase,and death phase.Growth curve of bacteria1.Lag Phase 2.Exponential Phase 3.Stationary Phase4.Death Phase Lag Phase When a microbial population is inoculated into a fresh medium,growth usually does not begin immediately but only
11、after a period of time called the lag phase,which may be brief or extended depending on the history of the culture and growth conditions.This happens because for growth to occur in a particular culture medium the cells must have a complete complement of enzymes for synthesis of the essential metabol
12、ites not present in that medium.Exponential Phase It is a consequence of the fact that each cell divides to form two cells,each of which also divides to form two more cells,and so on.Most unicellular microorganisms grow exponentially,but rates of exponential growth vary greatly.In general,prokaryote
13、s grow faster than eukaryotic microorganisms If a single bacterium continued to grow exponentially for 48 hr,produce a population that weighed about 4000 times the weight of Earth!This is particularly impressive because a single bacterial cell weighs only about one-trillionth(10 l2)of a gram.Station
14、ary PhaseAn essential nutrient of the culture medium is used up or some waste product of the organism builds up in the medium to an inhibitory level and exponential growth ceases,or both.If incubation continues after a population reaches the stationary phase,the cells may remain alive and continue t
15、o metabolize,but they may also die.If the latter occurs,the population is said to be in the death phase.Death Phase Population growth is measured by following changes in the number of cells or weight of cell mass.7.3 Measurement of Growth The number of cells in a population can be measured by counti
16、ng a sample under the microscope,either on samples dried on slides or on samples in liquid.With liquid samples,special counting chambers must be used.Total Cell CountDirect microsopic counting procedure using the Petroff-Hausser counting chamber.The usual practice,which is the most valid statistical
17、ly,is to count colonies only on plates that have between 30 and 300 colonies.To make a 10-fold(101)dilution,one can mix 0.5 ml of sample with 4.5 ml of diluent,or 1.0 ml sample with 9.0 ml diluent.Viable Counting methodThe usual way to perform a viable count is to determine the number of cells in th
18、e sample capable of forming colonies on a suitable agar medium.There are two ways of performing a plate count:the spread plate method and the pour plate method.In either case the sample must usually be diluted before plating.The number of colonies obtained in a viable count depends not only on the i
19、noculum size but also on the suitability of the culture medium and the incubation conditions used;It also depends on the length of incubation.The length of incubation.Some tiny colonies may be missed during the counting.The incubation conditions(medium,temperature,time).Key dilutions must be prepare
20、d.Sources of Error in Plate Counting A cell suspension looks cloudy(turbid)to the eye because cells scatter light passing through the suspension.The more cells present,the more light scattered and hence the more turbid the suspension.Turbidimetric Measurements of Cell Number A continuous culture is
21、essentially a flow system of constant volume to which medium is added continuously and from which continuous removal of any overflow can occur.Once such a system is in equilibrium,cell number and nutrient status remain constant,and the system is said to be in steady state.7.4 Continuous Culture:The
22、Chemostat The most common type of continuous culture device used is a chemostat,which permits control of both the population density and the growth rate of the culture.Both parameters can be set by the experimenter.The ChemostatChemostat used for continuous cultures.Rate of growth can be controlled
23、either by controlling the rate at which new medium enters the growth chamber or by limiting a required growth factor in the medium.Continuous culture of microorganismsRelationship among nutrient concentration,growth rate(solid line),and growth yield(dashed line)in a batch culture(closed system).At l
24、ow nutrient concentrations both growth rate and growth yield are affected.Steady-state relationships in the chemostat.The dilution rate is determined from the flow rate and the volume of the culture vessel.Thus,with a vessel of 1000ml and a flow rate through the vessel of 500ml/hr,the dilution rate
25、would be 0.5hr-1.Note that at high dilution rates,growth cannot balance dilution,and the population washes out.Note also that although the population density remains constant during steady state,the growth rate(doubling time)can vary over a wide range.Thus,the experimenter can obtain populations wit
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