I
(See Section 2(1))Part-A Specifications of Bio Fertilisers1. Nitrogen Fixing Bio-Fertilisers: -
A. Rhizobium Inoculants (RI) (IS 8268 - 2001)(i)RI shall be carried based the colour depending on the colour of the carrier(ii)RI shall contain a minimum of 10(7) viable Rhizobium cells/g of the carrier on dry - mass basis till 6 months expiry period from the date of manufacture. The number shall be counted by the plate count method as given in 4.2 and 4.3 of 1A of Part B of Schedule-II.(iii)RI shall have a maximum of six months expiry period from the date of manufacture.(iv)RI shall have no contamination with other micro-organisms at 10(5) dilution when counted as given in 4.3 of 1 A of Part B of Schedule- II.(v)The pH of RI shall be between 6.5 and 7.5 when tested as given in Annexure-A.(vi)RI shall show effectiveness nodulation on all those species and / or cultivars on the packet before the expiry date when tested. If good effectiveness pink nodulation is obtainable in the inoculated species together with total absence or sometimes presence of stray nodules in the controls, it should be concluded that RI contains effective Rhizobium the total dry mass of inoculated plants shall be significantly higher than that of the un-inoculated controls and at least 50 percent more than the controls.(vii)The carrier material such as peat, lignite, peatsoil, humus favouring growth to be neutralized with calcium carbonate and sterilized shall be in the form of a powder capable of passing through 150 to 212 micron (72 to 100 mesh) IS sieve.(viii)Specified mother culture be obtained from any recognized institution maintaining the mother cultures. The manufacturer may control the quality of the broth, it should get verified at least by two institutions as mentioned below:Note. - At present National Bio-fertiliser Development center and (NBDC), Ghaziabad and its Six Regional Centres located at Bangalore, Bhubaneshwar, Imphal, Hissar, Jabalpur and Nagpur, Indian Agricultural Research Institute (IARI), New Delhi, Tamil Nadu Agricultural University (TNAU) Coimbatore, University of Agricultural Science, Bangalore are sources for supplying the mother culture.(ix)The RI carrier shall be in the form of fribal (moist) with 30-40 percent (m/ m) moisture content when tested as given in Annex-B.(B)Azotobacter Chroococcum Inoculants (AI) (IS 9138 -2002)(i)AI shall be carrier- based, the colour depending on the colour of the carrier.(ii)AI shall contain a minimum of 10(7) viable Azotobacter cell/g of the carrier on dry - mass basis till 6 months expiry period from the date of manufacture. The number shall be counted by the plate count method as given in 4.2 of 1 A of Para B of Schedule II and Azotobactor Chroococcum colonies are gummy, raised with or without striations, viscous and often sticky. The pigmentation varies from very light brown to black. Count the colony number and observe the cyst formation as given Part B - Schedule II (4.2) and calculate number per gram of the carrier material.(iii)AI shall have a maximum of six months expiry period from the date of manufacture.(iv)AI shall have no contamination with other microorganisms at 10(5) dilution.(v)The pH of AI shall be between 6.5 and 7.5 when tested as given in -A.(vi)The carrier material such as peat, lignite, peatsoil, humus favouring growth to be neutralized with calcium carbonate and sterilized shall be in the form of a powder capable of passing through 150 to 212 micron (72 to 100 mesh) IS sieve.(vii)Specified mother culture be obtained from any recognized institution maintaining the mother cultures. The manufacturer may control the quality of the broth, it should get verified atleast by two institutions as mentioned in VIII of 1 of Part A of Schedule -I.(viii)The AI carrier shall be in the form of fribal (moist) with 30-40 percent (m/ m) moisture content when tested as given in Annexure-BC. Azospirillum Inoculants (ASI) (IS 14806-2000)(i)ASI shall contain 10(7) viable Azospirillum cells / g of the carrier material on dry mass basis.(ii)ASI shall no contamination with other microorganisms at 10(5) dilution. ASI contamination in semi solid medium should be checked by semi dilution and spread plate method with solid complete medium.(iii)The pH of ASI shall be 6.5 to 7.5 when tested as given in Annexure-A(iv)The ASI carrier shall be in the form of fribal (moist) with 30-40 percent moisture. When tested as given in Annexure-B(v)ASI shall show effective root development on all cultivars/crops against which the Inoculant is intended to be used.(vi)Specified mother culture be obtained from any institution maintaining the mother cultures. The manufacturer may control the quality of the both, it should get verified atleast by two institutions as mentioned in VIII of I of past A of schedule-I.2. Phosphate Solubilising Bacterial Inoculant (PSBI) (IS 14807-2000)
(i)PSIB shall contain 10(7) available phosphate solubilising bacterial cells / g of the carrier material on dry mass basis.(ii)PSBI shall be carrier based colour depending on the colour of the carrier. Carrier material such as peat, lignite charcoal may be used. It shall be neutralized with calcium carbonate and then sterlised. When tested it shall pass through 100 micron sieve.(iii)PSBI shall have no contamination with other microorganisms at 10(5) dilution.(iv)The pH of PSBI shall be 6.5 to 7.5.(v)The PSBI carrier shall be in the form of fribal (moist) with 30-40 percent (m/m) moisture content when tested as given in Annexure-B.(vi)PSBI shall have phosphate solubilising capacity in the range of minimum 30 percent in terms of zone formation minimum 30 percent in terms of zone formation minimum 10 mm solubilisation zone in a prescribed solid having at least 3 mm thickness. When tested by the method prescribed in Annexure-C.(vii)Specified mother culture be obtained from any recognized institution maintaining the mother culture. The manufacturer may control the quality of broth, it should get verified at least by two institutions mentioned in VIII of I of Part A of schedule-I.
I
Part B – Packing Marking and Storage
1. Packing. - RI shall be packed material of low density polyethylene / polypropylene bags thickness of which shall be 75-100 micron minimum.
2. Marking. - Each packet shall be marked legibly to give the following information:
(i)Name of the product, specifically as Rhizobium inoculant(ii)Leguminous crop for which intended(iii)Name and address of the manufacturer(vii)Date of expiry (agreed between the manufacturer and the purchaser subject to minimum 6 months from the date of manufacture)(viii)Net quantity and the area meant for(ix)Storage instructions worded as under: STORE IN COOL PLACE AWAY FROM DIRECT SUN AND HEAT'(x)Any other information.3. Item (ii), (vi) and (vii) shall be printed on a colour ink background
4. Directors for the use of RI shall be printed brief on the packet as given in - Annexure D. A separate pamphlet may preferably be given with it.
5. The product may also be marked with the standard mark
6. The use of the standard mark in governed by the provisions of the Bureau of Indian Standards Act 1986 and the rules and regulations made there under. The details of conditions under which the license for the use of the standard Mark may be granted to manufacturers or producers may be obtained from the Bureau of Indian Standards.
7. RI shall be stored by the manufacturer in a cool and dry place away from direct heat preferably at a temperature of 15 C to 30 C. It shall also be the duty of the manufacture to instruct the retailers and. in turn the users about the precautions to be taken during storage.
1. Packing. - AI shall be packed in packaging material of low density polythene / polypropylene bags thickness of which shall be 75-100 micron minimum.
2. Marking. - Each packet shall be marked legibly to give the following information.
(a)Name of the product, specifically as Azotobactor inoculant;(b)Non-leguminous crop for which intended(c)Name and address of the manufacturer(f)Date of expiry (agreed between the manufacturer and the purchaser subject to minimum 6 months from the date of manufacture)(g)Net quantity and rate of application.(h)Storage instructions worded as under Store in Cool Place Away From Direct Sun and Heat(i)Any other information.3. Direction for the use of AI shall be printed briefly on the packet as given in Annexure-D. A separate pamphlet may preferably be given with it.
4. The product may also be marked with the standard mark.
5. The use of the standard mark is governed by the provisions of the Bureau of lndian Standards Act, 1986 and the rules and regulations made there under. The details of conditions under which the license for the use of standard mark may be granted to manufacturers or producers may be obtained from the Bureau of Indian Standards.
6. AI shall be stored by the manufacturer in a cool and dry place away from direct heat preferably at a temperature of 15°C to 30°C. It shall also be the duty of the manufacturer to instruct the retailers and, in turn the users about the precautions to be taken during storage.
1. Packing. - ASI shall be packed in polyethylene packs, thickness which shall not be less than 75-100 micron.
2. Marking. - Each polyethylene packs shall be marked legibility and indelibly with the following information.
(a)Name of the product, specially as Azospirillium inoculant.(b)Name and address of the manufacturer(c)Crop (S) for which intended(d)Type of the carrier used.(g)Expiry date which shall not be less than months from the date of manufacture(h)Net mass in kg and area meant for;(i)Storage instructions worded as under: STORE IN COOL PLACE AWAY FROM DIRECT SUNLIGHT AND HEAT.(j)Any other information required under the Standards of Weights and Measures (packaged commodities) Rules 19773. Direction for use of ASI shall be printed briefly on the packets as given in Annexure -D of the standard. A separate pamphlet may preferable by given with it.
4. The product may also be marked with the Standard Mark.
5. The use of the Standard Mark is governed by the provisions of Bureau of Indian Standards Act, 1986 and rules and regulations made there under. The details of conditions under which the license for the use of standard mark may be granted to manufacturer or producers may be obtained from the Bureau of Indian Standards.
6. ASI shall be stored by the manufacturer in a cool and dry place away from direct heat preferably at a temperature of 20°C and not exceeding 30°C. It shall also be the duty of the manufacturer to instruct the retailers and, in turn, the users about the precautions to be taken during storage.
4. Phosphates Solublising Bacterial Inoculant (PSBI)
1. Packing. - PSBI shall be packed in polyethylene packs, thickness of which shall not be less than 100 micron.
2. Marking. - Each polyethylene packs shall be marked legibly and indelibly with the following information.
(a)Name of the product, specially as Phosphate solubilising bacterial inoculant;(b)Name and address of the manufacturer.(c)Crop (S) for which intended(d)Type of the carrier used.(g)Expiry date which shall not be less than 6 months from the date of manufacture(h)Net mass in kg and area meant for;(i)Storage instructions worded as under. - Store In Cool Place Away From Direct Sunlight and Heat.3. Direction for use of PSBI shall be printed briefly on the packets as given in Annexure-D of the standard. A separate pamphlet may preferably be given with it.
4. The product may also be marked with the Standard Mark.
5. The use of the Standard Mark is governed by the provisions of Bureau of Indian Standards Act, 1986 and rules and regulations made there under. The details of conditions under which the license for the use of standard mark may be granted to manufacturer or producer may be obtained from the Bureau of Indian Standards.
6. PSBI shall be stored by the manufacturer in cool and dry place away from direct heat preferably at a temperature of 20°C and not exceeding 30°C. It shall also be the duty of the manufacturer to instruct the retailers and in turn the users about the precautions to be taken during storage.
II
Part-A (See Section 21)Procedure for Sampling of Biofertilisers1. General Requirements. - 1.0. In drawing, preparing and handling the samples, following precautions and direction shall be observed.
1.1Sampling shall be carried out by a trained and experienced person as it is essential that the sample should be representative of the lot to be examined.1.2Since the samples are also required for micro biological analysis, utmost care is necessary to avoid extraneous contamination while drawing and handling the samples and to preserve them in their original conditions till they are ready for examination in the laboratory.1.2.1. No preservation or bacteriicidal/ fungicidal agent shall be added to samples required for micro-biological analysis.1.3Simples in their original up opened packets should be drawn and sent to the laboratory. This will prevent possible contamination of the samples during handling and also help in revealing the true conditions of the material.1.4Intact packets shall be drawn from a protected place not exposed to dampness, air, light, dust or soot and transferred to clean containers.1.5The sampling appliances and sample containers shall be sterile.1.6All precautions shall be taken to protect the sample the material being sampled, the sampling instruments and the sample container against adventitious contamination at the time of drawing the sample, opening containers and transferring the samples.2. Sample Equipment. - 2.1. A suitable scoop made of stainless steel may be used for drawing samples.
2.2The sampling equipment shall be perfectly clean and sterile. It shall be properly sterlised by heating in a hot air oven at 160°C for not less than 2 h or by autoclaving for not less than 20 min at 120°C and held in suitable containers to prevent recontamination.3. Scale of Sampling. - 3.1. Lot
All units (containers in a single consignment of type of material belonging to the same batch of manufacture) shall constitute a lot. If a consignment consists of different batches of the manufacture the containers of the same batch shall be separated and shall constitute a separate lot.3.2Batch. - An inoculant prepared from a batch fermentor or a group of flasks (containers) constitute a batch.3.3For ascertaining conformity of the material to the requirements of the specification, samples shall be tested from each lot separately.3.4The number of packets to be selected from a lot shall depend on the size of the lot and these packets shall be selected at random and in order to ensure the randomness of selection.4. Drawl of samples. - Three(3) samples should be drawn separately from each lot as per 1.3 of part A of schedule-11. One sample should be sent for analysis, one has to be handed over to the dealer under acknowledgement, and one will be treated as referee sample.
4.2The samples should be put in a cloth bag which may be sealed as specified in From K along with other details like sample no. / code no. which enables its identification.
II
Part-B (See Section 22)1. A. Method of Analysis of Rhizobium Bio-Fertilisers
1. Apparatus. - 1.1. Pipettes Graduated 1 ml and 10 ml
1.2Dilution Bottles or Flasks1.3Petri Dishes Clear, Uniform, flat-bottomed.1.4Hot - Air Oven Capable of giving uniform and adequate temperature equipped with a thermometer, calibrated to read up to 250 C and with vents suitably located to assure prompt and uniform heating.1.7Hand Tally or Mechanical counting Device2. Reagents. - 2.1. Congo Red and one percent aqueous solution
2.2MediumUse a plating medium of the following composition
| Agar |
20 g |
| Yeast Extract |
1 g |
| Mannitol |
10 g |
| Potassium hydrogen phosphate (K2HP04) |
0.5 g |
| Magnesium sulphate (MgS04 7H20) |
0.2 g |
| Sodium Chloride (NaCL) |
0.1 g |
| Congo red |
2.5 ml |
| Distilled water |
1000 ml |
| PH |
7.0 |
3.
l. Sterlise the sampling and plating equipment with diy heat in a hot air oven at not less than 160°C for not less than 2 hours.2.3.2. Sterlise the media by autoclaving at 120°C for 20 min. To permit passage of steam into and from closed containers when autoclaved, keep stoppers slightly loosened. Air from with in the chamber of the sterlise should be ejected allowing steam pressure to rise.Preparation of Plating Medium and Pouring2.3.3. Prepare growth medium in accordance with the composition indicated in 2.2.2.3.4. Melt the required amount of medium in boiling water or by exposure to following steam in partially closed container but avoid prolonged exposure to unnecessarily high temperature during and after melting. Melt enough medium which will be used with in 3h.Re-sterlisation of the medium may cause partial precipitation of ingredients.2.3.5. When holding time is les than 30 min, promptly cool the melted medium to about 45°C, and store until used, in a water bath or incubator at 43 to 45°C. introduce 12 to 15 ml of liquefied medium or appropriate quantity depending on size of the petridish at 42 to 44°C into each plate. Gently lift the cover of the dish just enough to pour in the medium, Sterlise the lips of the medium containers by exposure to flame.a. immediately before pouring.b. periodically during pouring, andc. when pouring is complete for each batch of plates, if portions of melted medium remain in containers and are to be used without subsequent and are to be used without subsequent sterilization for pouring additional plates. As each plate is poured thoroughly mix the medium with test portions in the Petri dish.2.3.6. By rotating and tilting the dish and without splashing the medium over edge, spread the medium evenly over the bottom of the plate. Provided conditions so that the medium solidifies with reasonable promptness (5-10 min) before removing the plates from level surface.3. Preparation of Serial Dilutions for Plate Counts. - 3.1. Dispense 30 g of Inoculant to 270 ml of sterile distilled or demineralized water and shake for 10 min on a reciprocal shaker or homogeniser. Make serial dilutions up to 10 (10) Take 0.2 ml or suitable aliquots of 10(6) to 10 (9) dilutions using sterile pipette and deliver to Petri dishes containing set medium as given in 2.1 and spread it uniformly. Invert the plates and promptly place them in the incubator.
4. Incubation of Plates. - Label the plates and incubate at 28 +/-2°C for 3 to 5 days for fast growing Rhizobia and 5 to 10 days slow growing ones
4.2Colony Counting aids.Count the colonies with the aid of magnifying lens under uniform and properly controlled artificial illumination. Use a colony counter, equipped with a guide plate and rules in centimeter square. Record the total number of colonies with the hand tally. Avoid mistaking particles of un-dissolved medium or precipitated matter in plates for pin-point colonies. The distinguish colonies form dirt, specks and other foreign matter, examine doubtful objects carefully.4.3Count all plates but consider for the purpose of calculation plates showing more than 30 and less than 300 colonies per plate. Disregard colonies which absorb Congo red and stand out as reddish colonies. Rhizobium stands out as white, translucent, glistening and elevated colonies. Count such colony numbers and calculate figures in terms of per liter, of carrier. Also check for freedom from contamination at 10 (8) dilution.1. B. Method of Analysis of Azotobactor Bio-Fertiliser
1. Apparatus - same as 1 of 1A of part B of schedule-II.
2. Reagents. - 2.1. Medium
Use a plating medium of the following composition
| Agar |
20 g |
| Sucrose (C12 H2 Ol 1) |
20.0 g |
| Ferric sulphate (Fe2 (S04)2) |
0.1 g |
| Dibasic potassium phosphate (K2HP04) |
1.0 g |
| Magnesium sulphate (MgS04, 7H20) |
0.5 g |
| Sodium Chloride (NaCl) |
0.5 g |
| Calcium carbonate (CaC02) |
2.0 g |
| Sodium Molybdate (Na2 MO 04) |
0.005 gm |
| Distilled water 1000 ml |
pH 6.8 to 7.2 |
3. Preparation of Serial Dilutions for Plate Counts. - Dispense 30 g of Inoculant to 270 ml of sterile distilled water and shake for 10 min on a reciprocal shaker. Make serials dilutions up to 1010Take 0.2 ml or suitable aliquots of 106 to 109 dilutions using sterile pipettes and deliver to Petri dishes containing set medium as given in 2.1 and spread it uniformly. Invert the plates and promptly place them in the incubator.
4. Incubation of Plates. - 4.1. Label the plates and incubate at 28+/ - 3°C for 4 to 6 days.
4.2Colony counting aidsSame as 4.2 of 1 A of Part B of Schedule-IIAzotobactor chrococcum colonies are gummy raised with or without striations, viscous and often sticky. The pigmentation varies from very light brown to black. Count the colony number and observe the cyst formation as given below and calculate number per grant of the carrier material.Grow the vegetative cells at 30 C on Burks agar medium comprising sucrose 20 g, dipotassium hydrogen phosphate 0.64 g, dihydrogen potassium phosphate 0.20 g; sodium chloride 0.20 g; calcium sulphate 0.05 g, sodium molybdate 0.001 g; ferric sulphate 0.003 g. agar 20 g and distilled water 1.000 ml. Look for vegetative cells after 18 to 24 h either by simple staining method or through a phase contrast microscope.Grow the cyst cells on Burks agar medium as given above with 0.3 percent n-butanol in place of the carbon source. Look for cyst formation after 4 to 5 days incubation.1.
C. Method of Analysis of Azospirillum Bio-Fertiliser1. Apparatus. - same as 1 A of Part B of schedule II
2. Reagents. - 2.1. Medium
Use a plating medium of the following composition
| Malic acid |
5.0 g |
| Potassium hydroxide |
4.0 g |
| Di-potassium hydrogen phosphate |
0.5 g |
| Ferrous sulphate |
0.05 g |
| Manganese sulphate |
0.01 g |
| Magnesium sulphate |
0.1 g |
| Sodium chloride |
0.2 g |
| Calcium chloride |
0.1 g |
| Sodium Molybdate |
0.002 g |
| Distilled water |
1000ml |
| Boromothymol blue (0.5% alcoholic solution) |
2.0 m. |
| Agar |
1.7 g |
| PH adjusted to |
6.5 - 7.0 |
3. Preparation Of Serial Dilutions for Plate Counts. - Same as IB of part B of schedule-II
4. Incubation of Plates. - 4.1. Label the plates and incubate at 28+/ - 3°C for 4 to 6 days.
4.2Colony counting aids: Same as 4.2 of 1 A of part B of schedule-IICountingCounting the tubes or plates which have turned blue in colour after inoculation and ascertain the presence of pellicles in undisturbed medium. To determine usual contamination on the same examine doubtful objects carefully.Count all plates/ tubes which have turned blue and consider them for the purpose of calculation. Count such type of tubes/ plates and tally this court with MPN table Annexure-E to get the number of cells per gram of the carrier.| Azospirillum Count/g of carrier =| MPN table value x Dilution levelDry mass of product |
1. Apparatus. - same as 1 A of Part B of schedule-I
2. Reagents. - 2.1. Medium
Use a plating medium of the following composition:
| Glucose |
10.0 g |
| Tri-calcium phosphate |
5.0 g |
| Ammonium sulphate |
0.5 g |
| Magnesium sulphate |
0.1 g |
| Sodium Chloride |
0.2 g |
| Yeast extract |
0.5 g |
| Manganese sulphate |
Trace |
| Ferrous sulphate |
Trace |
| Distilled water |
1000 ml |
| Agar |
15.0 g |
| PH adjusted to 7 +/- 0.2 |
|
3. Preparation of Serial Dilution for Plate Counts. - Same as 1 B of part B of schedule-II
4. Incubation of Plates. - 4.1. Label the plates and incubate at 28+/ - 3°C for 4 to 6 days.
4.2Colony counting aids: Same as 4.2 of 1 A of part B of schedule - IICountingCount the total number of colonies on the plates including colonies with solubilisation zone with the help of a colony counter.Methods for counting solubilisation zones. - (a) Take 10 g of PSBI (BF) in 90 ml in water(b)Make a ten fold dilution series up to 107(c)Take 0.2 ml aliquote of 105 to 107 dilution using sterile pipettes and delivered to Petri dishes containing pikowskeyi media.(d)Spread it uniformly, Invert the plates and incubate them up to 2 weeks at 28+/- 2°C.(e)Count the colonies showing hallow cones and measure their diameter. Minimum acceptable zone is 10 mm in diameter.Guidelines of Maintenance and Preparation of Culture and Quality Control at Broth Stage.1. Maintenance of pure cultures. - 1.1. Maintain pure cultures of rhizobia on yeast extract mannitol agar (YEMA) slants of the following composition.
| Mannitol |
10.0 g |
| Potassium hydrogen phosphate (k2HP04) |
0.5 g |
| Magnesium sulphate (MgS04 7H20) |
0.2 g |
| Sodium chloride (NaCl) |
0.1 g |
| Calcium Carbonate (Ca C03) |
1.0 g |
| Yeast extract |
1.0 g |
| Agar |
18.0 g |
| Distilled water |
1 liter |
| pH |
6-8-7.0 |
2. Preparation of Inoculum Cultures
2.1Prepare yeast monnitol broth of the composition as given in 1.1. minus the agar.2.2Transfer a loopfull of the culture into a 100/250 ml conical flasks containing the broth. Incumbate the flasks at 28+- 2°C on the rotary shaker for 2 to 6 days.4. Quality Control Tests Recommended at Broth Stage. - 4.1. Qualitative Tests
4.1.1. Check for freedom from visible contaminants4.1.2. The pH of the bacterial broth shall normally be between 6.5 and 7.54.1.3. Smear and Gram stain4.1.3.1. Reagentsa. Ammonium oxalate crystal violet stain weigh 0.2 g of crystal violet and dissolve in 20 ml of 95 percent ethyl alcohol. Dissolve separately 0.8 g of ammonium oxalate in 80 ml of distilled water. Mix the two solutions and fitter through a filter paper.b. Iodine solution
| Iodine |
1.00 g |
| Potassium Iodide |
2.00 g |
| Distilled water |
300 ml |
| Erythrosine |
1.00 g |
| Phenol |
5.00 g |
| Distilled water |
100 ml |
| Glucose |
10.0 g |
| Peptone |
20.0 g |
| Sodium chloride (NaCI) |
5.0 |
| Agar (IS 6850} |
15.0 |
| Distilled water |
1000 ml |
| Bromocresol purple |
10 ml of |
| ethyl alcohol solution |
1.6 persons |
| pH |
7.2 |
1. Maintenance of pure cultures.
1.1Maintain pure cultures of Azotobactor on slants of the following composition
| Agar |
20 gm |
| Sucrose |
20 gm |
| Ferric Sulphate |
0.1 |
| Dibasic Potassium Phosphate |
1.0 gm |
| Magnesium Sulphate |
0.5 gm |
| Calcium carbonate |
2.0 gm |
| Sodium Molybdate |
0.005 gm |
| Distilliled water |
1000 ml |
| PH |
6.8 to 7.2 |
2. Preparation of inoculum culture. - 2.1 Prepare Jonsons media broth of the composition as given in 1.1. minus the agar
2.2Transfer a loop full of the culture into 100ml/250 ml, conical flask containing the broth. Incubate the flasks at 28 +/- 2°C on a rotary shaker for 2 to 6 days.3. Quality control Tests recommended at broth stage.
3.1Qualitative test. - 3.1.1 Check for free from contaminants by preparing slide and observing under microscope.3.1.2The pH by bacterial broth shall normally be between 6.5 to 7.03.1.3Gram staining test shall be carried out as described in 4.1.3, 4.1.3.1 and 4.1.3.2 of Rhizobium of this standard.3.2Quantitative test3.2.1. Viable cell count: same as 4.2. of IB of part B of Schedule II1. Maintenance of pure cultures. - 1.1. Maintenance of pure cultures of Azospirillum on nitrogen free bromothymol blue medium and maintain as semi solid medium as described in 2.1 of this standard 1C of part B of Schedule II
1.2Transfer a loopful of pure culture to each of the agar culture tube aseptically in an inoculation room and incubate 28 +/- 2°C for three days and keep in undisturbed.Always keep pure culture below 5°C.2. Preparation of Inoculum culture. - Inoculum culture shall be prepared as described in 2.1, 2.2 of Rhizobium of this standard. ,,
3. Quality Control Test recommended at Broth Stage
3.1Qualitative Test3.1.1. Check for free from contaminants by preparing slide and observing under microscope.3.1.2. The pH of bacterial broth shall normally be between 6.5 to 7.0.3.1.3. Gram staining test shall be carried out as described in 4.1. 3., and 4.1.3.1 & 4.1.3.2. of Rhizobium of this standard.3.1.4. See the colour change in the media after 24 hours from inoculation. The colour will change from green to blue.3.1.5. Watch the pellicle just below the surface of the media. It checked on the third day after keeping inoculated broth undisturbed.3.2Quantitative Test3.2.1. Most Probable Number (MPN) as given in Annexure-E. The counts of Azosprillium in the final broth from shake culture or fermentors shall be not less than 108 to 109 cells / ml. Other wise the broth should be rejected.4. Phosphate Solubilizing Bacterial Inoculant (PSBI)
1. Maintenance of pure cultures. - 1.1. Maintain pure culture of PSBI on the medium as described in 2.1 of 1 D of part B of schedule- II in the form of slants
1.2Transfer a loopful of pure culture to each of the agar slants aseptically in an inoculation room and incubate at 28 + /- 2°C for three days. Always keep pure culture below 5°C.2. Preparation of Inoculum culture. - Inoculum culture shall be prepared as described in 2.1, 2.2. of Rhizobium changing the media composition as mentioned in 2.1 of this standard.
3. Quality control test reo amended at Broth Stage. - 3.1. Qualitative Test
3.1.1. Check for free from visible contaminants by microscope and observing solubilisation zones.3.1.2. The pH of bacterial broth shall normally be between 6.5 to 7.0.3.1.3. Gram staining test shall be carried out as described in 4.1.3,4.1.3.1, and 4.1.3.2 of Rhizobium.3.2Quantitative Test3.2.1Viable cell count serially dilute one milli liter of broth plate 0.2. ml aliquots of the dilutions on pikowkyasi media (as given in 2.1 of 1 D of Part B of Schedule II) plates and incubate at 28 +/- 2°C for 2 to 6 days. The counts of PSBI in the final broth from shake culture or fermentors shall be not less than 108 to 109 cells/ml. Otherwise, the broth should be rejectedAnnexure-ADetermination of PH1. Make suspension of 20 g of the ASI into 50 ml of distilled water and shake on a rotary shaker for 2 hours. Filter this suspension and determine the pH of the filterate with the held of pH meter.
Annexure-BDetermination of Moisture of Bio-Fertiliser Packets (Method)2.1Heat 10 g of sample for 12-16 hours in an air over at 100-105°C, in desiccator and weigh. The loss in weight represents the moisture. Calculate the moisture percentage on air dry weight basis, by multiplying the loss in weight by ten.Annexure-CDetermination of Soluble Phosphorus Using Ascorbic Acid.Principle. - Soluble phosphorus from hetropoly molybdophosphate complex with molybdate ions which on reduction produces blue colour measured at 840 to 880 nm. Considering the higher stability of the ascorbic acid, easiness to handle, higher tolerance to the concentration of interfering ions, possibilities to use it with all type of acids and higher stability of the developed colour (10 to 60 min), ascorbic acid instead of stannous chloride is now - a-days used as the reducing agent for the hetropoly molybdophosphate complex formed by the soluble phosphate ions on addition of ammonium molybdate solution.apparatus. - Spectrophotometer capable of transmission measurements at 840 to 880 nm.Reagents. - Ammonium Molybdate1. - Ascorbic acid
P - Nitrophenol
Preparation of Reagents. - Sulphomolybdic acid.Take 20 g of Ammonium molybdate and dissolve in 300 ml of distilled waterAdd slowly 450 ml of 10 N2 S04.Cool the above mixture and add 100 ml of 0.5 percent solution of Antimonypotassium tartrate.Cool and make the volume to one litre. Store in glass bottle away from direct sunlight.Preparation of mixed Reagent. - Add 1.5 gm of L - ascorbic acid in 100 ml of the above stock solution and mix. Add 5 ml of this solution to develop colour. Mixed regent is to be prepared fresh as it does not keep for more than 24 h.Procedure. - Weigh the required material in a 100 ml conical flask.Add 50 ml of extractant and shake it for 30 min on rotary shaker.Filter the suspension through whatman filter paper No. 40. If the filterate is coloured than add a tea spoon of Darco-60 (activated phosphorus free carbon) reshake and filter.Take a known aliquot (5 to 25 ml) of the extract in a 50 ml volumetric flask.Add 5 drops of P-nitrophenol indicator (1.5 percent solution in Water) and adjust the pH of the extract between 2 and 3 with the help of NH2S04. The yellow colour will disappear when the pH of the solution becomes 3. Swirl gently to avoid loss of the solution along with the evolution of C04.When the C02 evolution has subsided. Wash down the neck of the flask and dilute the solution to about 40 ml.Add 5 ml of the sulphomolybdic acid mixed reagent containing ascorbic acid Swril the content and make up the volume.Measure the transmission after 30 min. at 880 nm using red filter. The blue colour developed remains stable up to 60 minutes.Record the concentration of Phosphorus (P) in the extract from the standard curve and calculate the concentration of soluble phosphorus as follows.Calculation. - (a) Weight of the substance taken = xg(b)Volume of the extractant added=50 ml(c)Volume of the extract taken for p=y ml determination.(d)Volume made after colour developed = 50 ml(e)Reading from the standard curve = z ppm against percent transmission recorded.| Percent p =| ZX50X10 -6X5O X 100Y,X |
1. The contents of the packet are sufficient for seeds to be sown in the area indicated on the package.
2. Use only for the leguminous crops mentioned, before the expiry date and do not expose to direct sun light or heat.
3. Mix the inoculants with the seeds gently with the minimum amount of water, taking care to avoid damage to seed coat. Dry the inoculated seeds under shade over clean paper or gunny bag and sow immediately.
This is not a chemical fertiliser and hence do not mix inoculated seeds or RI with chemical fertilisers.Azotobactor1. Use only for the non-leguminous crops and before the expiry date.
2. The contents of the packet are sufficient for seeds to be sown in 0.4 hectare.
3. This is not a chemical fertilizer, hence do not mix it or the inoculated planting material with chemical fertilizers or pesticides.
4. Use for the crops specified on the packet.
5. Do not expose to direct sunlight or heat.
Azospirillum1. The contents of the packet are sufficient enough to the given area to be broadcasted or given seedlings for root dipping depending on the specified crops as denoted in the packet. Mix the inoculants with seeds gently with the minimum amount of water, taking care to avoid damage to seed coat. Dry the inoculated seed under shade over clean surface gunny bag and sow them immediately.
2. Use only for the crops mentioned paddy, Azospirillum brasillense for other crops like millets, etc use crop specific strain. Use before the expiry date and do expose to direct sun light or heat.
3. ASI is not a chemical fertilizer hence do not mix inoculated seeds or ASI with agrochemicals.
Phosphate Solubilising Bacteria.1. The contents of the packet are sufficient enough to the given area to be broadcast or given seedlings for root dipping depending on the specified crops as denoted on the packet. Mix the inoculants with seeds gently with the minimum amount of water, taking care to avoid damage to seed cost. Dry the inoculated seed under shade over clean dry paper organic bag and sow them immediately.
2. In order to solubilise fixed soil phosphate use PSBI for all type of crops. Use before the expiry date and do not expose to direct sunlight or heat.
3. PSBI is not chemical fertiliser hence do not mix inoculated seeds or PSBI with agrochemicals.
