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ISOLATION OF Rhizobium.pdf

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Nistarini College, Purulia (W.B) India

This PowerPoint Presentation intends to explore the isolation of Rhizobium and the contribution of microbes to soil fertility on a large scale.

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General account about the microbes used as biofertilizer – Rhizobium – isolation, identification, mass multiplication, carrier based inoculants, Actinorrhizal symbiosis.
A Presentation by Dr. N. Sannigrahi, Associate Professor, Department of Botany, Nistarini College, Purulia, D.B. Road, Purulia (W.B) India-723101
 Microbes are the tiny, invisible biological world observed under magnifying devices-microscope, ultra microscope like SEM etc.  They include single- and multi-celled organisms, both prokaryotes and eukaryotes can be microorganisms. They can be bacteria, archaea, fungi, or protists.  We can only see up to 100 micrometers (µm) with our bare eyes, so organisms smaller than this size are considered microorganisms (Fig. 1).  Microorganisms are found in every ecosystem and can also be closely associated with many multicellular organisms.  Bacteria are single-celled prokaryotic microorganisms that can live freely or in association with a host and are omnipresent within our environment. When bacteria are said to be omnipresent, it means that they are present in virtually every habitat on Earth, from the soil to the ocean to within our bodies. Bacteria even inhabit seemingly inhospitable environments, such as within the hot soil in and near volcanoes and in radioactive waste.
 Archaea are another type of single-celled prokaryotic organism and, until relatively recently, were believed to be another kind of bacteria known as archaebacteria. This is due to the many similarities that archaea and bacteria share.  Fungi are eukaryotic organisms that can be microscopic or visible. Perhaps the fungi you are most familiar with are mushrooms since they are visible to the naked eye (and, sometimes, edible)!  Despite the physical appearance of mushrooms, fungi are not plants and are, instead, members of a separate biological kingdom unique from animals and plants. For our purposes, we are only interested in microscopic fungi, known as micro fungi.  Protists are mostly microscopic, single-celled organisms, including algae species, amoebas, ciliates, slime molds, and more. Protists appear to be a very diverse group of organisms, and protist taxonomy is mainly in a state of flux due to continually changing classifications and discoveries.  All the microbe4s play a number of beneficial; & harmful attributes and the functions can be summarized as below:
 Bacteria play a vital role in our environment and within our bodies. The presence of bacteria is essential for all other life on Earth.  Bacteria are both decomposers and producers - they decompose dead organic matter and waste into inorganic matter rich in nutrients, thus allowing plants to grow. These plants then feed herbivores, which in turn feed carnivores.  Inside and on animals, including humans, bacteria can be found as part of the micro biome, playing vital roles such as aiding digestion. In fact, disruption of the micro biome is believed to play a role in developing specific syndromes and diseases. While most bacteria are harmless or beneficial to humans, some can cause illness, disease, and even death. These are known as pathogenic bacteria.  They can act as the decomposers and to be used as the fertilizers of biological origin. Some of the bacteria have the potential to act as bio- fertilizers.  Some of the fungi play a very significant role and acts as the fertilizers with the close association of the higher plants- the symbiotic assessment is considered as mycorrhizae.
 Rhizobium is a genus of bacteria belongs to Rhizobiaceae family acclaimed for its ability to institute mutualism with leguminous plants and ultimately fix elemental dinitrogen. With the furtherance of research, Rhizobium has gained expeditious traction because of which legume–Rhizobium technology has also risen to popularity. Amid such advancement, hydroponics is being applied to screen symbiotic interactions of Rhizobium in order to obtain more information on their genetic and molecular mechanisms including functionality in the host plant. The bacteria enter the roots of leguminous plants and create nodules, within which molecular nitrogen is reduced to ammonia, which is then used by the plant to synthesize vitamins, proteins, and other nitrogen-containing substances. As a result, these root nodules serve as ammonium-ion storage sites (Flores-Félix et al., 2013). Rhizobium increases growth in non-leguminous crops by changing their root shape and growth physiology. Furthermore, Rhizobium spraying boosts crop productivity by increasing plant height, seed germination, nitrogen content, and leaf chlorophyll (Sara et al., 2013). Rice seed inoculation with various Rhizobium strains at increasing levels of nitrogen increases the content of straw by 4%–19% and the yield of rice grain by 8%– 22% (Sammauria et al., 2020). Rhizobia include bacteria such as Rhizobium, Bradyrhizobium , Azorhizobium, Mesorhizobium, and Sinorhizobium etc.
 Rhizobium are symbiotic diazotrophs,  A gram (-) soil bacteria endo-symbiotic association with legumes,  Rod shaped non-spore forming bacteria,  Invade legume root through root hairs,  Form effective red colored LHb in the root nodules and fix atmospheric nitrogen,  5 important genera- Rhizobium-slow-growing rhizobia forms acid, Bradyrhizobium-fast –growing alkali, Azorhizobioum infects both stem & root, Sinorhiozobium ,Photorhizobium,  Different Rhizobium grows on different hosts like R. leguminosorum on pea, R. phaseoli of Bean, R. trifoli on Clover, R. meliloti on alfa-alfa, R. japonicum on soyabean, R. lupine on lupine groups.  Most of the cases, the basic nature of the infections and the developmental stages are almost identical and the multiplication in large steps are almost identical.
Name of the group of host plant Name of Rhizobium Sp. Name of the host plant Nitrogen fixation.kg/ year Pea Group R. leguminosorium Pea ( Pisum sativum), Lentil ( Lens culinaris) 62-132 Soybean Group R. Japonica Soybean ( Glycine max) 57-105 Lupine Group R. lupini Lupinus arcticus 70-90 Alfalfa group R. meliloti Melilotus indicus 100-150 Beans Group R. phaseoli Phaseolus munga 80-110 Clover group R. trifolii Trifolium repens 130 Cowpea Group R. species Cicer arietinum, Phaseolus munga 57-105
 Healthy nodules were isolated from the six month old D. sissoo seedlings grown under net house conditions.  The nodules were washed in tap water to remove the adhering soil particles on its surface.  Nodules were dipped in 0.1 % mercuric chloride (HgCl2) solution for 30 second and then washed successively eight to ten times with sterilized distilled water to remove the traces of HgCl2.  Surface sterilized nodules were crushed in sterilized distilled water by glass rod to obtain a milky suspension of bacteriods.  The suspension was streaked on YEMA medium and incubated at 28±2°C for 2-5 days.  The growth on YEMA medium was counted and expressed as cfu/g. Isolates obtained from nodules of Dalbergia sissoo were purified on YEMA medium by streak plate method  Authentication Congo red test All the purified rhizobial isolates were streaked on CRYEMA medium and were observed for absorption of Congo red dye (Vincent, 1970).
 Bromothymol blue test The YEMA medium containing bro-mothymol blue was streaked with isolated strains and was observed either for yellow color due to production of acids or blue color due to production of alkali (Norris, 1965).  Hofer’s alkaline test This test is based on the fact that Rhizobium is unable to grow at higher pH 11.0 on yeast extract mannitol broth (Hofer, 1935). Ketolactose agar test: Ketolactose agar plates were streaked with isolated microbes. After incubation for 4-6 days at 28±2°C, the plates were flooded with Benedict’s solution. This test is based on the fact that Rhizobium is unable to utilize the lactose (Bernaerts and Deley, 1963).  Plant infection test The different isolates were tested for their ability to nodulate Dalbergia sissoo plants grown in plastic pots. Seeds of Dalbergia sissoo were inoculated with Rhizobium isolates by soaking seeds. Plants were carefully uprooted after 75 days and observed for nodulation.
 The multiplication of the Rhizobium is very important for the large scale inoculation of the microbes in the host tissue to improve the plant health by making the avenues accessible to the standing crops . Only the inoculums of this particular species is not enough, it also needs the addressing of the processing along with the packaging for transportation from the laboratory to the fields.  The mass production of Rhizobium comprises the following steps for the successful multiplication of the microbes in the large scale:  Inoculums preparation,  Processing of carrier material,  Selection of ideal carrier material,  Preparation of carrier material,  Mixing the carrier & broth culture and packing,  Preparation of the inoculants packing.
 The inoculums preparation needs the preparation before the process and it needs the in depth knowledge about the microbial pure culture techniques garnished with the following apparatuses-  Autoclave for sterilization- for making the media & glass goods along with desired materials contamination free  Hot air oven- Growth of the microbes at desired temperature  Laminar Air Flow chamber- Transfer of inoculums in aseptic environment  Incubator- Incubation of the microbes  Rotary and Shaker- Aeration of the growth of the microbes  pH meter- To maintain the desired pH of the microbes  Refrigerator- To preserve the inoculants at low temperature  Fermentor- A large vessel for mass production of microbes in controlled condition  In addition to these, the media preparation along with the desired growth materials and continuous electric supply is essential in order to maintain the aseptic environment for the successful execution of the entire microbiological process.
 INOCULUMS PREPARATION:  The inoculums preparation needs the understanding of the following features of the isolation of the Rhizobium from the root nodules.  Materials Required: Roots of the Legume plants, sterile distilled water, pipettes, test tubes, YEMA plates, 70% ethanol, 0.1% Mercuric chloride solution, aseptic conditions by using the disinfectants and sterilizing materials along with the basic ingredients of the microbiological attributes.  1. The root nodules are collected, washed with the running tap water and treated with 0.1% mercuric chloride or 3-5% Hydrogen peroxide,  2.After repeated running with the tap water, the nodules are passed through 70% ethyl alcohol,  YEMA plates are prepared with the sterilized environment,  1 gm of nodular extract is prepared with 10 ml of distilled water and mixed properly,  Serial dilution is made up to 10-8
 Suspension of 0.1 ml from 10-8 is taken and poured over the plates prepared previously and made it, spreads throughout the plate,  In the suitable environmental conditions at 32℃ is incubated for further analysis.  PREPARATION OF STOCK CULTURE  After incubation, after 4-5 days, the Rhizobium colony will appeared on the plate and it is identified with congored dye . Most of the Rhizobium colony arte white in color and took the stain of congored.  The colony took the strain are Rhizobium,  The pH of the stock culture to be kept at 6.8.  For large scale production, production of starter culture is required; the starter culture is prepared in suitable broth,  In the starter culture, the conical flasks are kept at the suitable temperature for the same in the large scale production.
 PRODUCTION OF CARRIER BASED INOCULUM  After the production of semi-liquid inoculums from the fermentor, the carrier materials are taken,  The carrier materials may be pit, lignite, vermiculite, charcoal of the farmyard manure,  The carrier materials must be cheap, easily available, low toxic contents along with high organic contents to address the economic feasibility,  Water holding capacity of the carrier materials must be more than 50%,  The carrier materials must be transformed into dust and the pH must be maintained with calcium carbonate powder,  The all sorts of material to be autoclaved properly for making the substances free from the contamination.  The carrier materials must have some adhesive property so as to hold with the root surface where the inoculation to be exercised
 PACKING:  During the packaging, the bacterial culture must be kept in a metallic tray with the suitable carrier and with the help of mixture or using hand gloves, the mixture must be mixed properly before storage,  The suitable measure to be adopted for the proper sterilization to do the procedure for the optimum benefit that to be expected in this consequences.  The polythene bags should be low density grade with a thickness of 50-75 micron,  The package should contain the following information- the name of the manufacturer, name of the strain, the crop which to recommended along with the method of inoculation, date of manufacturer, date, batch number, price etc,  Full address of the manufacturer along with storage,  Instructions to the farmers for its uses and application
 STORGAE OF BIO-FERTILIZER PACKET  The packets should be stored in a cool place far from the heat & sunlight,  The packets should be stored in room temperature or in cold storage conditions in lots in plastic crates or the gunny bags,  The population of the inoculants must be checked at the 15 days interval for its optimum utilization,  There should be more than 10 to the power 9 inoculants at the time of packaging and 10 to the power 7 inoculants at the time of disposal,
 The term "actinorhiza" refers both to the filamentous bacteria Frankia, an actinomycete, and to the root location of nitrogen-fixing nodules. Actinorhizal plants are classified into four subclasses, eight families, and 25 genera comprising more than 220 species. Although ontogenically related to lateral roots, actinorhizal nodules are characterized by differentially expressed genes, supporting the idea of the uniqueness of this new organ. Two pathways for root infection have been described for compatible Frankia interactions:  root hair infection or intercellular penetration. Molecular phylogeny groupings of host plants correlate with morphologic and anatomic features of actinorhizal nodules. Four clades of actinorhizal plants have been defined, whereas Frankia bacteria are classified into three major phylogenetic groups. Although the phylogenies of the symbionts are not fully congruent, a close relationship exists between plant and bacterial groups.
 A model for actinorhizal specificity is proposed that includes different levels or degrees of specificity of host-symbiont interactions, from fully compatible to incompatible. Intermediate, compatible, but delayed or limited interactions are also discussed. Actinorhizal plants undergo feedback regulation of symbiosis involving at least two different and consecutive signals that lead to a mechanism controlling root nodulation.  These signals mediate the opening or closing of the window of susceptibility for infection and inhibit infection and nodule development in the growing root, independently of infection mechanism.
 Soil fertility & soil health are important for crop productivity.  The natural restoration of soil fertility is the call of the time due to eutrophication and soil quality deterioration,  The different microbes in general and some bacteria, BGA and fungi in particular play a very significant role in this regard,  Free living bacteria Azotobacter & clostridium etc play important role to fix atmospheric nitrogen,  Different symbiotic produce root nodules and the actively fox nitrogen by Rhizobiun leguminosarum produce nodule in the legume plants,  By means of biochemical process, the atmospheric free nitrogen are fixed by the symbiotic mechanisms,  Bacteria like Frankia fix nitrogen in association with angiosperms like Alnus, Casuarina etc  The huge demand of biofertilizers in the context of organic farming is increasing day to day and the production of bio-fertlizers can be done by the process of industrial process,  The isolation followed by large scale production, packaging and to transport to the fields are very important in this context.
 References:  1. Fundamental Botany- Sen & Giri  2. A text of Fungi- Vasistha,  3. A Textbook of Microbiology- R.P. Singh,  4.Textbook of Microbiology- Dubey & Maheswari  5. Soil Microbiology- N.S. Subba Rao  6. Agricultural Microbiology- G. Rangaswami  7. Google for images  8. Different WebPages for information.  Disclaimer: This PPT has been made to enrich free online study resources without any pleasure of financial interest.

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ISOLATION OF Rhizobium.pdf

  • 1. General account about the microbes used as biofertilizer – Rhizobium – isolation, identification, mass multiplication, carrier based inoculants, Actinorrhizal symbiosis.
  • 2.
  • 3. A Presentation by Dr. N. Sannigrahi, Associate Professor, Department of Botany, Nistarini College, Purulia, D.B. Road, Purulia (W.B) India-723101
  • 4.  Microbes are the tiny, invisible biological world observed under magnifying devices-microscope, ultra microscope like SEM etc.  They include single- and multi-celled organisms, both prokaryotes and eukaryotes can be microorganisms. They can be bacteria, archaea, fungi, or protists.  We can only see up to 100 micrometers (µm) with our bare eyes, so organisms smaller than this size are considered microorganisms (Fig. 1).  Microorganisms are found in every ecosystem and can also be closely associated with many multicellular organisms.  Bacteria are single-celled prokaryotic microorganisms that can live freely or in association with a host and are omnipresent within our environment. When bacteria are said to be omnipresent, it means that they are present in virtually every habitat on Earth, from the soil to the ocean to within our bodies. Bacteria even inhabit seemingly inhospitable environments, such as within the hot soil in and near volcanoes and in radioactive waste.
  • 5.  Archaea are another type of single-celled prokaryotic organism and, until relatively recently, were believed to be another kind of bacteria known as archaebacteria. This is due to the many similarities that archaea and bacteria share.  Fungi are eukaryotic organisms that can be microscopic or visible. Perhaps the fungi you are most familiar with are mushrooms since they are visible to the naked eye (and, sometimes, edible)!  Despite the physical appearance of mushrooms, fungi are not plants and are, instead, members of a separate biological kingdom unique from animals and plants. For our purposes, we are only interested in microscopic fungi, known as micro fungi.  Protists are mostly microscopic, single-celled organisms, including algae species, amoebas, ciliates, slime molds, and more. Protists appear to be a very diverse group of organisms, and protist taxonomy is mainly in a state of flux due to continually changing classifications and discoveries.  All the microbe4s play a number of beneficial; & harmful attributes and the functions can be summarized as below:
  • 6.  Bacteria play a vital role in our environment and within our bodies. The presence of bacteria is essential for all other life on Earth.  Bacteria are both decomposers and producers - they decompose dead organic matter and waste into inorganic matter rich in nutrients, thus allowing plants to grow. These plants then feed herbivores, which in turn feed carnivores.  Inside and on animals, including humans, bacteria can be found as part of the micro biome, playing vital roles such as aiding digestion. In fact, disruption of the micro biome is believed to play a role in developing specific syndromes and diseases. While most bacteria are harmless or beneficial to humans, some can cause illness, disease, and even death. These are known as pathogenic bacteria.  They can act as the decomposers and to be used as the fertilizers of biological origin. Some of the bacteria have the potential to act as bio- fertilizers.  Some of the fungi play a very significant role and acts as the fertilizers with the close association of the higher plants- the symbiotic assessment is considered as mycorrhizae.
  • 7.
  • 8.  Rhizobium is a genus of bacteria belongs to Rhizobiaceae family acclaimed for its ability to institute mutualism with leguminous plants and ultimately fix elemental dinitrogen. With the furtherance of research, Rhizobium has gained expeditious traction because of which legume–Rhizobium technology has also risen to popularity. Amid such advancement, hydroponics is being applied to screen symbiotic interactions of Rhizobium in order to obtain more information on their genetic and molecular mechanisms including functionality in the host plant. The bacteria enter the roots of leguminous plants and create nodules, within which molecular nitrogen is reduced to ammonia, which is then used by the plant to synthesize vitamins, proteins, and other nitrogen-containing substances. As a result, these root nodules serve as ammonium-ion storage sites (Flores-Félix et al., 2013). Rhizobium increases growth in non-leguminous crops by changing their root shape and growth physiology. Furthermore, Rhizobium spraying boosts crop productivity by increasing plant height, seed germination, nitrogen content, and leaf chlorophyll (Sara et al., 2013). Rice seed inoculation with various Rhizobium strains at increasing levels of nitrogen increases the content of straw by 4%–19% and the yield of rice grain by 8%– 22% (Sammauria et al., 2020). Rhizobia include bacteria such as Rhizobium, Bradyrhizobium , Azorhizobium, Mesorhizobium, and Sinorhizobium etc.
  • 9.
  • 10.  Rhizobium are symbiotic diazotrophs,  A gram (-) soil bacteria endo-symbiotic association with legumes,  Rod shaped non-spore forming bacteria,  Invade legume root through root hairs,  Form effective red colored LHb in the root nodules and fix atmospheric nitrogen,  5 important genera- Rhizobium-slow-growing rhizobia forms acid, Bradyrhizobium-fast –growing alkali, Azorhizobioum infects both stem & root, Sinorhiozobium ,Photorhizobium,  Different Rhizobium grows on different hosts like R. leguminosorum on pea, R. phaseoli of Bean, R. trifoli on Clover, R. meliloti on alfa-alfa, R. japonicum on soyabean, R. lupine on lupine groups.  Most of the cases, the basic nature of the infections and the developmental stages are almost identical and the multiplication in large steps are almost identical.
  • 11.
  • 12. Name of the group of host plant Name of Rhizobium Sp. Name of the host plant Nitrogen fixation.kg/ year Pea Group R. leguminosorium Pea ( Pisum sativum), Lentil ( Lens culinaris) 62-132 Soybean Group R. Japonica Soybean ( Glycine max) 57-105 Lupine Group R. lupini Lupinus arcticus 70-90 Alfalfa group R. meliloti Melilotus indicus 100-150 Beans Group R. phaseoli Phaseolus munga 80-110 Clover group R. trifolii Trifolium repens 130 Cowpea Group R. species Cicer arietinum, Phaseolus munga 57-105
  • 13.
  • 14.  Healthy nodules were isolated from the six month old D. sissoo seedlings grown under net house conditions.  The nodules were washed in tap water to remove the adhering soil particles on its surface.  Nodules were dipped in 0.1 % mercuric chloride (HgCl2) solution for 30 second and then washed successively eight to ten times with sterilized distilled water to remove the traces of HgCl2.  Surface sterilized nodules were crushed in sterilized distilled water by glass rod to obtain a milky suspension of bacteriods.  The suspension was streaked on YEMA medium and incubated at 28±2°C for 2-5 days.  The growth on YEMA medium was counted and expressed as cfu/g. Isolates obtained from nodules of Dalbergia sissoo were purified on YEMA medium by streak plate method  Authentication Congo red test All the purified rhizobial isolates were streaked on CRYEMA medium and were observed for absorption of Congo red dye (Vincent, 1970).
  • 15.  Bromothymol blue test The YEMA medium containing bro-mothymol blue was streaked with isolated strains and was observed either for yellow color due to production of acids or blue color due to production of alkali (Norris, 1965).  Hofer’s alkaline test This test is based on the fact that Rhizobium is unable to grow at higher pH 11.0 on yeast extract mannitol broth (Hofer, 1935). Ketolactose agar test: Ketolactose agar plates were streaked with isolated microbes. After incubation for 4-6 days at 28±2°C, the plates were flooded with Benedict’s solution. This test is based on the fact that Rhizobium is unable to utilize the lactose (Bernaerts and Deley, 1963).  Plant infection test The different isolates were tested for their ability to nodulate Dalbergia sissoo plants grown in plastic pots. Seeds of Dalbergia sissoo were inoculated with Rhizobium isolates by soaking seeds. Plants were carefully uprooted after 75 days and observed for nodulation.
  • 16.
  • 17.  The multiplication of the Rhizobium is very important for the large scale inoculation of the microbes in the host tissue to improve the plant health by making the avenues accessible to the standing crops . Only the inoculums of this particular species is not enough, it also needs the addressing of the processing along with the packaging for transportation from the laboratory to the fields.  The mass production of Rhizobium comprises the following steps for the successful multiplication of the microbes in the large scale:  Inoculums preparation,  Processing of carrier material,  Selection of ideal carrier material,  Preparation of carrier material,  Mixing the carrier & broth culture and packing,  Preparation of the inoculants packing.
  • 18.  The inoculums preparation needs the preparation before the process and it needs the in depth knowledge about the microbial pure culture techniques garnished with the following apparatuses-  Autoclave for sterilization- for making the media & glass goods along with desired materials contamination free  Hot air oven- Growth of the microbes at desired temperature  Laminar Air Flow chamber- Transfer of inoculums in aseptic environment  Incubator- Incubation of the microbes  Rotary and Shaker- Aeration of the growth of the microbes  pH meter- To maintain the desired pH of the microbes  Refrigerator- To preserve the inoculants at low temperature  Fermentor- A large vessel for mass production of microbes in controlled condition  In addition to these, the media preparation along with the desired growth materials and continuous electric supply is essential in order to maintain the aseptic environment for the successful execution of the entire microbiological process.
  • 19.  INOCULUMS PREPARATION:  The inoculums preparation needs the understanding of the following features of the isolation of the Rhizobium from the root nodules.  Materials Required: Roots of the Legume plants, sterile distilled water, pipettes, test tubes, YEMA plates, 70% ethanol, 0.1% Mercuric chloride solution, aseptic conditions by using the disinfectants and sterilizing materials along with the basic ingredients of the microbiological attributes.  1. The root nodules are collected, washed with the running tap water and treated with 0.1% mercuric chloride or 3-5% Hydrogen peroxide,  2.After repeated running with the tap water, the nodules are passed through 70% ethyl alcohol,  YEMA plates are prepared with the sterilized environment,  1 gm of nodular extract is prepared with 10 ml of distilled water and mixed properly,  Serial dilution is made up to 10-8
  • 20.  Suspension of 0.1 ml from 10-8 is taken and poured over the plates prepared previously and made it, spreads throughout the plate,  In the suitable environmental conditions at 32℃ is incubated for further analysis.  PREPARATION OF STOCK CULTURE  After incubation, after 4-5 days, the Rhizobium colony will appeared on the plate and it is identified with congored dye . Most of the Rhizobium colony arte white in color and took the stain of congored.  The colony took the strain are Rhizobium,  The pH of the stock culture to be kept at 6.8.  For large scale production, production of starter culture is required; the starter culture is prepared in suitable broth,  In the starter culture, the conical flasks are kept at the suitable temperature for the same in the large scale production.
  • 21.  PRODUCTION OF CARRIER BASED INOCULUM  After the production of semi-liquid inoculums from the fermentor, the carrier materials are taken,  The carrier materials may be pit, lignite, vermiculite, charcoal of the farmyard manure,  The carrier materials must be cheap, easily available, low toxic contents along with high organic contents to address the economic feasibility,  Water holding capacity of the carrier materials must be more than 50%,  The carrier materials must be transformed into dust and the pH must be maintained with calcium carbonate powder,  The all sorts of material to be autoclaved properly for making the substances free from the contamination.  The carrier materials must have some adhesive property so as to hold with the root surface where the inoculation to be exercised
  • 22.  PACKING:  During the packaging, the bacterial culture must be kept in a metallic tray with the suitable carrier and with the help of mixture or using hand gloves, the mixture must be mixed properly before storage,  The suitable measure to be adopted for the proper sterilization to do the procedure for the optimum benefit that to be expected in this consequences.  The polythene bags should be low density grade with a thickness of 50-75 micron,  The package should contain the following information- the name of the manufacturer, name of the strain, the crop which to recommended along with the method of inoculation, date of manufacturer, date, batch number, price etc,  Full address of the manufacturer along with storage,  Instructions to the farmers for its uses and application
  • 23.  STORGAE OF BIO-FERTILIZER PACKET  The packets should be stored in a cool place far from the heat & sunlight,  The packets should be stored in room temperature or in cold storage conditions in lots in plastic crates or the gunny bags,  The population of the inoculants must be checked at the 15 days interval for its optimum utilization,  There should be more than 10 to the power 9 inoculants at the time of packaging and 10 to the power 7 inoculants at the time of disposal,
  • 24.  The term "actinorhiza" refers both to the filamentous bacteria Frankia, an actinomycete, and to the root location of nitrogen-fixing nodules. Actinorhizal plants are classified into four subclasses, eight families, and 25 genera comprising more than 220 species. Although ontogenically related to lateral roots, actinorhizal nodules are characterized by differentially expressed genes, supporting the idea of the uniqueness of this new organ. Two pathways for root infection have been described for compatible Frankia interactions:  root hair infection or intercellular penetration. Molecular phylogeny groupings of host plants correlate with morphologic and anatomic features of actinorhizal nodules. Four clades of actinorhizal plants have been defined, whereas Frankia bacteria are classified into three major phylogenetic groups. Although the phylogenies of the symbionts are not fully congruent, a close relationship exists between plant and bacterial groups.
  • 25.  A model for actinorhizal specificity is proposed that includes different levels or degrees of specificity of host-symbiont interactions, from fully compatible to incompatible. Intermediate, compatible, but delayed or limited interactions are also discussed. Actinorhizal plants undergo feedback regulation of symbiosis involving at least two different and consecutive signals that lead to a mechanism controlling root nodulation.  These signals mediate the opening or closing of the window of susceptibility for infection and inhibit infection and nodule development in the growing root, independently of infection mechanism.
  • 26.
  • 27.  Soil fertility & soil health are important for crop productivity.  The natural restoration of soil fertility is the call of the time due to eutrophication and soil quality deterioration,  The different microbes in general and some bacteria, BGA and fungi in particular play a very significant role in this regard,  Free living bacteria Azotobacter & clostridium etc play important role to fix atmospheric nitrogen,  Different symbiotic produce root nodules and the actively fox nitrogen by Rhizobiun leguminosarum produce nodule in the legume plants,  By means of biochemical process, the atmospheric free nitrogen are fixed by the symbiotic mechanisms,  Bacteria like Frankia fix nitrogen in association with angiosperms like Alnus, Casuarina etc  The huge demand of biofertilizers in the context of organic farming is increasing day to day and the production of bio-fertlizers can be done by the process of industrial process,  The isolation followed by large scale production, packaging and to transport to the fields are very important in this context.
  • 28.  References:  1. Fundamental Botany- Sen & Giri  2. A text of Fungi- Vasistha,  3. A Textbook of Microbiology- R.P. Singh,  4.Textbook of Microbiology- Dubey & Maheswari  5. Soil Microbiology- N.S. Subba Rao  6. Agricultural Microbiology- G. Rangaswami  7. Google for images  8. Different WebPages for information.  Disclaimer: This PPT has been made to enrich free online study resources without any pleasure of financial interest.