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WELCOME TO
MY
INTERNSHIP PRESENTATION
Presented by
Abu Musa
Exam Roll: 2030
Registration no: 2015817772
Department of Fisheries
University of Dhaka
1
2
Topic
Summary
Introduction
Materials and Methods
Results
Conclusion and Recommendation
The Outline of Presentation
3
 pH, salinity, temperature and DO respectively in the study area were 6.5, 26.5 ppt, 30.7 ℃ and
3.4 ppm over the study period.
 The total number of identified genera of phytoplankton and zooplankton was 11.
 The density of plankton was 167 individuals per cubic meter seawater.
Summary
4
The small and microscopic organisms drifting or floating in the sea or fresh water, consisting chiefly of
diatoms, protozoans, small crustaceans, and the eggs and larval stages of larger animals.
-Oxford Dictionary
Definition of Plankton
Introduction
01 Phytoplankton
Phytoplankton are the autotrophic (self-
feeding) components of the plankton
community and a key part of ocean and
freshwater ecosystems
02
Zooplankton
zooplankton consisting of small animals and
the immature stages of larger animals.
5
 Live food organisms include all plants (phytoplankton) and animals
(zooplankton) which are used in finfish and shellfish larval rearing
system.
 Live foods are able to swim in water column and are available to fish
and shellfish larvae thereby stimulate the feeding response (David
2003)
 Phytoplankton comprises the base of the food chain in the marine
environment.
Introduction
Figure 1 The central role of microalgae in mariculture
(Brown et al., 1989). Source :FAO 1996
Plankton as live feed?
1. Brown, M.R. 1991. The amino acid and sugar composition of 16 species of microalgae used in mariculture. Aquaculture, 145: 79-99.
2. David, A. B., 2003. Status of marine aquaculture in relation to live prey: past, present and future. In: Live feeds in marine aquaculture Josianne, G. S., and Lesley, A.M.
(Eds.). Blackwell publishing, UK, pp. 1-16
6
Table-1: Culturable genera or species as live feed
7
Introduction
Diatoms Flagellates Green algae Rotifers Copepods
Skeletonema
costatum
Isochrysis
galbana
Chlorella spp. Brachionus
plicatilis
Acartia
Thalassiosira
pseudonana
Tetraselmis
suecica
Nannochloropsis
spp
B. rotundiformis Pseudodiaptomus
Chaetoceros
gracilis
Monochrysis
lutheri
Apocyclopus
C. calcitrans Calanus
Specific objectives
 To learn plankton biodiversity along Cox’s Bazar coast.
 To learn techniques of plankton identification
 To learn assessment of plankton population and water quality parameter.
 To acquire knowledge about culture system of live feed
Objective of The Study
Overall objective
The overall objective of this study is to understand and asses the current condition of
plankton biodiversity in the Bay of Bengal, Cox’s Bazar and Learning culture technique of
live feed.
9
Bangladesh
Cox’s Bazar Sea
Beach
Bakkhali
Bangladesh
Fisheries Research
Institute, Marine
Fisheries &
Technology
Station, Cox’s
Bazar
Internship Period: 23/03/2021-08/03/2021 (14 days)
Materials and Methods
10
Study Area & Duration of Study:
pH Meter Slide
Seawater Refractometer
Vortex Machine
Incubator Micropipette Plankton Net Agar Compound Microscope Weight Machine
Materials used in the study
Autoclave Machine
11
Study Procedure
Sample collection
Sample are collected
from selected area
1
Recording
Physicochemical
Conditions of
Water
Physicochemical
Condition recorded
regularly
2
Identification of
Plankton
Identification are
done by
Compound
Microscope
3
Counting of
plankton
Counting plankton
using mathematical
formula
4
Stock Culture of
phytoplankton
A selected species
was cultured
5
12
Sample Collection
Sample collecting from Holiday Point
Sample collecting from Kolatoli Point
 Plankton samples were collected horizontally from four selected areas
using simple conical tow-net oblique, which mesh size is 40
micrometers.
 Sample were collected filtering 40 L seawater
 Sample was collected just before high tide.
 Sample collected from 2-meter depth of sea water.
13
sample under microscope
Observing sample
Identification of Plankton
14
 The identification was performed by using a compound microscope
(LEICA DM500 compound microscope).
 Depending on plankton size 10X, 40X and 100X magnification were
used.
 Identification was done with the help of following book: illustration of
the marine phytoplankton of Japan and the site diatoms.org.
15
Plankton were counted using following formula:
No. individuals/ m3 =
𝑉1×𝐶
𝑉2×𝑉3
,
Where,
C = number of organisms counted,
V1 = volume of the concentrated sample (ml),
V2 = volume of the sample counted (ml),
V3 = volume of the filtered volume of water (m3)
Counting of plankton
Isolation of plankton
1
2
3
4
5
6
Isolation of
single cells
Serial dilution
Centrifuge
washing
technique
Preparation of
agar plat
Streak plating
technique
Enrichment
media
Solution (A)
1. Potassium Nitrate (KNO3) 100g
2. Sodium di-hydrogen orthophosphate
(NaH2PO4.2H2O)
20g
3. EDTA di-sodium salt (Na2EDTA) 45g
4. Boric Acid (H3BO3) 33.4g
5. Ferric Chloride (FeCl3) 1.3g
6. Manganous Chloride (MnCl2.2H2O) 0.36g
7. Distilled Water 1L
Solution (B)
1. Zinc Chloride (ZnCl2) 4.2g
2. Cobalt Chloride (CoCl2.6H2O) 4.0g
3. Copper Sulphate (CuSO4.5H2O) 4.0g
4. Ammonium molybdate ((NH4)6Mo7O24.4H2O) 1.8g
5. Distilled Water 1L
Solution (C)
1. Vitamin B1 (Thiamine) 2g
2. Vitamin B 12 (Cyanocobalamin) 100m
g
3. Distilled Water 1L
17
Enrichment media
 To grow skeletonema Conway/walne’s medium was used.
The media is prepared in lab using Conway/walne’s
formula.
 The nutrient media were put in each of the sampling bottles
in following amount 1ml of each Solution A, 0.5ml of B and
0.1 ml of C into 1 L sea water.
Parameters Used value Optimum
Temperature (°C) 25±1 18-24
Salinity (g L-1)
22-24 20-24
Light intensity (Lux) 2000-5000 2500-5000
Photoperiod Hrs. (light: dark) 24:0. 24:0 (max.)
pH 7.2 8.0-8.5 18
Stock Culture of phytoplankton
 The culture media of phytoplankton was prepared by washing 100 mL of conical flask and sterilized by using
autoclave for 15 min at 121EC.
 Required amount of Conway/walne’s and F2 medium were added.
19
Stock Culture of phytoplankton
Stock culture of Collected sample
Supplying nutrient media Culture Chamber
Isolation Unit
 The observation of culture done each day.
 After 2 days, when water colour was brown, the cell were counted by using a haemocytometer under
a compound micro-scope at 40X magnification
Culture Water Sterilization
Nutrient Enrichment
Inoculation Cell Count Stock Culture
Chlorination
Dechlorinated
Autoclave
Contaminated free live
organism
Wash by detergent
Wash by fresh water
Autoclave
Soaked in chlorine
Sodium nitrate, Sodium,
Hypophosphate,
Sodium silicate,
Ferric Chloride,
EDTA,
Thiamin,
Biotin
10% Inoculation
Using sprit lamp
Use 60% alcohol
Results (cell/ml)
Haemo-cytometer
Boiling
Removing bubble
Add Nutrient
Mixing sea water
and agar
Spreading species
20
Live feed Culture
Overall Procedure of Live feed Culture
Station pH Salinity Temperature DO
Laboni Point 6.5 32 25 3.7
Holiday Point 6.5 33 26 3.5
Kolatoli point 6.4 31 27 3.5
Fisheries
landing center,
Bakkhali
6.7 27 28 3.2
21
Results
 In this study, physicochemical conditions of water were
analysed.
 The average pH value is 6.5.
 The average salinity is 30.7
 Average temperature value is 26.5
 Average DO is 3.4
5
5.5
6
6.5
7
24-Feb 26-Feb 28-Feb 3-Mar 6-Mar
pH trend over the Study period
2
2.5
3
3.5
4
4.5
5
24-Feb 26-Feb 28-Feb 3-Mar 6-Mar
Trend of DO over the study period
22
Salinity and temperature
The pH was recorded each time after collecting sample from 4 different station and calculated average
value. The value of them shown in the chart-1
The DO of sea water was recorded each time after collecting sample. Calculation was done in lab. The
calculated value of DO is shown in the chart-2
Chart 1 pH trend over the Study period Chart 2 Trend of DO over the study period
28
29
30
31
32
33
34
35
24-Feb 26-Feb 28-Feb 3-Mar 6-Mar
Salinity trend over the study
period
24
25
26
27
28
29
30
24-Feb 26-Feb 28-Feb 3-Mar 6-Mar
Temperature trend over the
study period
23
Salinity and temperature
 The salinity was also recorded using a digital refractometer each time after collecting sample from 4 different
station and calculated average value. The value of them shown in the chart-3
 The Temperature of sea water was recorded each time after collecting sample. Calculation was done in lab. The
calculated value of DO is shown in the chart-4
Chart 3 salinity trend over the study period
Chart 3 Temperature trend over the study period
Class Order Family Genus
Eustigmatophyceae Eustigmatales Monodopsidaceae Nannochloropsis
Chaetocerotaceae Chaetoceros
Coscinodiscophyceae Skeletonema
Cyanophyceae Dinophysiales Dinophysiaceae Dinophysis
Bacillariophyceae Naviculales Naviculaceae Navicula
Bacillariophyceae Naviculales Pleurosigmataceae Gyrosigma
Cyanophyceae Spirulinales Spirulinaceae Spirilunia
Coscinodiscophyceae Rhizosoleniales Rhizosoleniaaceae Rhizosolenia
Hexanauplia Calanoida Acartiidae Acartia
Trebouxiophyceae Chlorellales Chlorellaceae Chlorella
Chlorodendrophyceae Chlorodendrales Chlorodendraceae Tetraselmis spp 24
Plankton Community
The total number of identified genera of plankton was 11 and many more unidentified in the Bay of Bengal
in following table
 Recommendations
After collecting sample, proper treatment should give to avoid death of plankton.
25
Conclusion and Recommendation
 Conclusion
The eleven genera had identified from the collected samples from mentioned coastal point. Among
them naocholoropsis , skeletonema, navivula and cholorella are important. Nannocholoropsis,
Cholorella. Skeletonema, Tetraselmis spp are used as live feed.
26

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Assessment of the Plankton Biodiversity, Bay of Bengal, Cox's Bazar, Bangladesh

  • 1. WELCOME TO MY INTERNSHIP PRESENTATION Presented by Abu Musa Exam Roll: 2030 Registration no: 2015817772 Department of Fisheries University of Dhaka 1
  • 3. Summary Introduction Materials and Methods Results Conclusion and Recommendation The Outline of Presentation 3
  • 4.  pH, salinity, temperature and DO respectively in the study area were 6.5, 26.5 ppt, 30.7 ℃ and 3.4 ppm over the study period.  The total number of identified genera of phytoplankton and zooplankton was 11.  The density of plankton was 167 individuals per cubic meter seawater. Summary 4
  • 5. The small and microscopic organisms drifting or floating in the sea or fresh water, consisting chiefly of diatoms, protozoans, small crustaceans, and the eggs and larval stages of larger animals. -Oxford Dictionary Definition of Plankton Introduction 01 Phytoplankton Phytoplankton are the autotrophic (self- feeding) components of the plankton community and a key part of ocean and freshwater ecosystems 02 Zooplankton zooplankton consisting of small animals and the immature stages of larger animals. 5
  • 6.  Live food organisms include all plants (phytoplankton) and animals (zooplankton) which are used in finfish and shellfish larval rearing system.  Live foods are able to swim in water column and are available to fish and shellfish larvae thereby stimulate the feeding response (David 2003)  Phytoplankton comprises the base of the food chain in the marine environment. Introduction Figure 1 The central role of microalgae in mariculture (Brown et al., 1989). Source :FAO 1996 Plankton as live feed? 1. Brown, M.R. 1991. The amino acid and sugar composition of 16 species of microalgae used in mariculture. Aquaculture, 145: 79-99. 2. David, A. B., 2003. Status of marine aquaculture in relation to live prey: past, present and future. In: Live feeds in marine aquaculture Josianne, G. S., and Lesley, A.M. (Eds.). Blackwell publishing, UK, pp. 1-16 6
  • 7. Table-1: Culturable genera or species as live feed 7 Introduction Diatoms Flagellates Green algae Rotifers Copepods Skeletonema costatum Isochrysis galbana Chlorella spp. Brachionus plicatilis Acartia Thalassiosira pseudonana Tetraselmis suecica Nannochloropsis spp B. rotundiformis Pseudodiaptomus Chaetoceros gracilis Monochrysis lutheri Apocyclopus C. calcitrans Calanus
  • 8. Specific objectives  To learn plankton biodiversity along Cox’s Bazar coast.  To learn techniques of plankton identification  To learn assessment of plankton population and water quality parameter.  To acquire knowledge about culture system of live feed Objective of The Study Overall objective The overall objective of this study is to understand and asses the current condition of plankton biodiversity in the Bay of Bengal, Cox’s Bazar and Learning culture technique of live feed. 9
  • 9. Bangladesh Cox’s Bazar Sea Beach Bakkhali Bangladesh Fisheries Research Institute, Marine Fisheries & Technology Station, Cox’s Bazar Internship Period: 23/03/2021-08/03/2021 (14 days) Materials and Methods 10 Study Area & Duration of Study:
  • 10. pH Meter Slide Seawater Refractometer Vortex Machine Incubator Micropipette Plankton Net Agar Compound Microscope Weight Machine Materials used in the study Autoclave Machine 11
  • 11. Study Procedure Sample collection Sample are collected from selected area 1 Recording Physicochemical Conditions of Water Physicochemical Condition recorded regularly 2 Identification of Plankton Identification are done by Compound Microscope 3 Counting of plankton Counting plankton using mathematical formula 4 Stock Culture of phytoplankton A selected species was cultured 5 12
  • 12. Sample Collection Sample collecting from Holiday Point Sample collecting from Kolatoli Point  Plankton samples were collected horizontally from four selected areas using simple conical tow-net oblique, which mesh size is 40 micrometers.  Sample were collected filtering 40 L seawater  Sample was collected just before high tide.  Sample collected from 2-meter depth of sea water. 13
  • 13. sample under microscope Observing sample Identification of Plankton 14  The identification was performed by using a compound microscope (LEICA DM500 compound microscope).  Depending on plankton size 10X, 40X and 100X magnification were used.  Identification was done with the help of following book: illustration of the marine phytoplankton of Japan and the site diatoms.org.
  • 14. 15 Plankton were counted using following formula: No. individuals/ m3 = 𝑉1×𝐶 𝑉2×𝑉3 , Where, C = number of organisms counted, V1 = volume of the concentrated sample (ml), V2 = volume of the sample counted (ml), V3 = volume of the filtered volume of water (m3) Counting of plankton
  • 15. Isolation of plankton 1 2 3 4 5 6 Isolation of single cells Serial dilution Centrifuge washing technique Preparation of agar plat Streak plating technique Enrichment media
  • 16. Solution (A) 1. Potassium Nitrate (KNO3) 100g 2. Sodium di-hydrogen orthophosphate (NaH2PO4.2H2O) 20g 3. EDTA di-sodium salt (Na2EDTA) 45g 4. Boric Acid (H3BO3) 33.4g 5. Ferric Chloride (FeCl3) 1.3g 6. Manganous Chloride (MnCl2.2H2O) 0.36g 7. Distilled Water 1L Solution (B) 1. Zinc Chloride (ZnCl2) 4.2g 2. Cobalt Chloride (CoCl2.6H2O) 4.0g 3. Copper Sulphate (CuSO4.5H2O) 4.0g 4. Ammonium molybdate ((NH4)6Mo7O24.4H2O) 1.8g 5. Distilled Water 1L Solution (C) 1. Vitamin B1 (Thiamine) 2g 2. Vitamin B 12 (Cyanocobalamin) 100m g 3. Distilled Water 1L 17 Enrichment media  To grow skeletonema Conway/walne’s medium was used. The media is prepared in lab using Conway/walne’s formula.  The nutrient media were put in each of the sampling bottles in following amount 1ml of each Solution A, 0.5ml of B and 0.1 ml of C into 1 L sea water.
  • 17. Parameters Used value Optimum Temperature (°C) 25±1 18-24 Salinity (g L-1) 22-24 20-24 Light intensity (Lux) 2000-5000 2500-5000 Photoperiod Hrs. (light: dark) 24:0. 24:0 (max.) pH 7.2 8.0-8.5 18 Stock Culture of phytoplankton  The culture media of phytoplankton was prepared by washing 100 mL of conical flask and sterilized by using autoclave for 15 min at 121EC.  Required amount of Conway/walne’s and F2 medium were added.
  • 18. 19 Stock Culture of phytoplankton Stock culture of Collected sample Supplying nutrient media Culture Chamber Isolation Unit  The observation of culture done each day.  After 2 days, when water colour was brown, the cell were counted by using a haemocytometer under a compound micro-scope at 40X magnification
  • 19. Culture Water Sterilization Nutrient Enrichment Inoculation Cell Count Stock Culture Chlorination Dechlorinated Autoclave Contaminated free live organism Wash by detergent Wash by fresh water Autoclave Soaked in chlorine Sodium nitrate, Sodium, Hypophosphate, Sodium silicate, Ferric Chloride, EDTA, Thiamin, Biotin 10% Inoculation Using sprit lamp Use 60% alcohol Results (cell/ml) Haemo-cytometer Boiling Removing bubble Add Nutrient Mixing sea water and agar Spreading species 20 Live feed Culture Overall Procedure of Live feed Culture
  • 20. Station pH Salinity Temperature DO Laboni Point 6.5 32 25 3.7 Holiday Point 6.5 33 26 3.5 Kolatoli point 6.4 31 27 3.5 Fisheries landing center, Bakkhali 6.7 27 28 3.2 21 Results  In this study, physicochemical conditions of water were analysed.  The average pH value is 6.5.  The average salinity is 30.7  Average temperature value is 26.5  Average DO is 3.4
  • 21. 5 5.5 6 6.5 7 24-Feb 26-Feb 28-Feb 3-Mar 6-Mar pH trend over the Study period 2 2.5 3 3.5 4 4.5 5 24-Feb 26-Feb 28-Feb 3-Mar 6-Mar Trend of DO over the study period 22 Salinity and temperature The pH was recorded each time after collecting sample from 4 different station and calculated average value. The value of them shown in the chart-1 The DO of sea water was recorded each time after collecting sample. Calculation was done in lab. The calculated value of DO is shown in the chart-2 Chart 1 pH trend over the Study period Chart 2 Trend of DO over the study period
  • 22. 28 29 30 31 32 33 34 35 24-Feb 26-Feb 28-Feb 3-Mar 6-Mar Salinity trend over the study period 24 25 26 27 28 29 30 24-Feb 26-Feb 28-Feb 3-Mar 6-Mar Temperature trend over the study period 23 Salinity and temperature  The salinity was also recorded using a digital refractometer each time after collecting sample from 4 different station and calculated average value. The value of them shown in the chart-3  The Temperature of sea water was recorded each time after collecting sample. Calculation was done in lab. The calculated value of DO is shown in the chart-4 Chart 3 salinity trend over the study period Chart 3 Temperature trend over the study period
  • 23. Class Order Family Genus Eustigmatophyceae Eustigmatales Monodopsidaceae Nannochloropsis Chaetocerotaceae Chaetoceros Coscinodiscophyceae Skeletonema Cyanophyceae Dinophysiales Dinophysiaceae Dinophysis Bacillariophyceae Naviculales Naviculaceae Navicula Bacillariophyceae Naviculales Pleurosigmataceae Gyrosigma Cyanophyceae Spirulinales Spirulinaceae Spirilunia Coscinodiscophyceae Rhizosoleniales Rhizosoleniaaceae Rhizosolenia Hexanauplia Calanoida Acartiidae Acartia Trebouxiophyceae Chlorellales Chlorellaceae Chlorella Chlorodendrophyceae Chlorodendrales Chlorodendraceae Tetraselmis spp 24 Plankton Community The total number of identified genera of plankton was 11 and many more unidentified in the Bay of Bengal in following table
  • 24.  Recommendations After collecting sample, proper treatment should give to avoid death of plankton. 25 Conclusion and Recommendation  Conclusion The eleven genera had identified from the collected samples from mentioned coastal point. Among them naocholoropsis , skeletonema, navivula and cholorella are important. Nannocholoropsis, Cholorella. Skeletonema, Tetraselmis spp are used as live feed.
  • 25. 26

Notas do Editor

  1. Good morning sir and madam. I am Abu Musa. Today I am presenting my internship presentation. Welcome to the presentation.
  2. My internship topic is
  3. This presentation are divided into Five sections. Moving to next section.
  4. Summary of the my internship programme. The average pH value is 6.5. The average salinity is 30.7 ppt Average temperature value is 26.5 C Average DO is 3.4 ppm Now we are move to second session- introduction
  5. What is plankton? Oxford dictionary defined plankton as There are two type of plankton. Phytoplankton are the autotrophic (self-feeding) components of the plankton community and a key part of ocean and freshwater ecosystems Zooplankton consisting of small animals and the immature stages of larger animals. Now we are moving to next slide.
  6. What is live feed? There a figure shown, role of microalgae in mariculture
  7. As live feed following species or genera are culture for different fish species. Under diatoms Class ……… species are include
  8. Gilthead seabream depend on Chorella sp species Lets move the next slide
  9. This slide is about Now we are going to third section
  10. This slide is about materials and methods The duration of internship period is 14 days The study location are shown in the map
  11. Here is The materials used for this study 1. plankton net for collecting sample 2. pH mater and seawater refractometer for recording physiochemical conditions 3.Microscope for identification 4.Vortex machine, autoclave, incubator for plankton isolation and culture ** Let's move to next slide
  12. This is a process flow chart of procedure. First step of Study procedure is stock culture of selected phytoplankton
  13. Now I am taking about sample collection After samples were collected samples were preserved in 25 mL plastic bottles with two conditions; in which, first containing 10% buffered formalin and second containing nutrient solution Conway / Walne’s medium. Samples with 10% formalin were used for species identification in the laboratory. Meanwhile, samples with nutrient solution to keep them alive for isolation and culture process. Let's scroll down to next slide.
  14. This slide is about Identification After collecting, these samples were brought to the live feed culture Laboratory BFRI, Cox’s Bazar for further analysis and identification. Sample were taken to slide to observe and identification Moving to next slide
  15. This slide about counting of plankton.
  16. Isolation of plankton are 6 steps process 1, A single cell of microalgae was picked from the sample using a micropipette under microscopic observation 2. The dilution factor is usually constant at each step, here I used 10 3.The sample tubes were centrifuged at 3000 rpm for 15 min. 5. The streak plating technique was performed under autoclave machine in axenic conditions.
  17. Nutritional requirements skeletonema depending on their natural habitat and cellular physiology.
  18. After that, the bottles were filled with 50 mL of distilled water. Parameter used for stock culture of skeletonema
  19. This slide is about stock culture of skeletonema
  20. 1st step is culture Culture water should be Sterilization can be done by For inoculation 60% alcohol used For cell counting hameo-cytometer is used Stock culture include …
  21. There is a table showing physiochemical conditions seawater of selected study area