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(New page: = Preservation of tissues for DNA analysis = ''(From: Dawson et al. 1998)'' === Equipment<br> === 1. Sterile syringes, forceps, dissecting scissors, or razor blades<br>2. A way of cl...)
 
 
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= Preservation of tissues for DNA analysis =
= Preservation of DNA  =


''(From: Dawson et al. 1998)''  
''(From: Dawson et al. 1998)''  


=== Equipment<br> ===
=== Equipment  ===


1. Sterile syringes, forceps, dissecting scissors, or razor blades<br>2. A way of cleaning the sampling tools if they are not disposable (e.g. flaming metal objects after dipping in ethanol, or a good rinse and wipe dry)<br>3. Vials containing 1-2 ml of preservative (DMSO+NaCl or ethanol [70% to 95%; &gt;90% preferred]; will be provided upon request).<br>4. Chest of ice (in the field); ice, refrigerator, or freezer (at lab/home, separate from food).<br>5. Protective gloves (latex, rubber)  
<br>1. Sterile syringes, forceps, dissecting scissors, or razor blades<br>2. A way of cleaning the sampling tools if they are not disposable (e.g. flaming metal objects after dipping in ethanol, or a good rinse and wipe dry)<br>3. Vials containing 1-2 ml of preservative (DMSO+NaCl or ethanol [70% to 95%; &gt;90% preferred]; will be provided upon request).<br>4. Chest of ice (in the field); ice, refrigerator, or freezer (at lab/home, separate from food).<br>5. Protective gloves (latex, rubber).<br>6. Waterproof paper.<br>7. Plastic bags and/or jars.<br>8. Plastic tray or container.


=== Procedure A <br> ===
=== Procedure A  ===


Sampling gut or gonad:<br>1. Collect medusae.<br>2. Starve the medusae for as long as possible.<br>3. Using a clean syringe, flush the guts with tapwater. Repeat several times to displace any debris from the guts.<br>4. Using the same syringe (or other tool), suck up (tear or cut) about 0.1-0.2 ml of gastric and/or gonadal tissues.<br>5. Preserve the tissue in one vial of preservative. (Make sure there is excess preservative; guard against diluting the preservative with too much water.)<br>6. Label the vial and put it on ice. Store on ice, in a freezer or refrigerator until the samples are shipped or analyzed (separate from food).<br>7. Clean tools and gloves, repeat for the next sample.  
<br>Sampling gut or gonad:<br>1. Collect medusae.<br>2. Starve the medusae for as long as possible.<br>3. Using a clean syringe, flush the guts with tapwater. Repeat several times to displace any debris from the guts.<br>4. Using the same syringe (or other tool), suck up (tear or cut) about 0.1-0.2 ml of gastric and/or gonadal tissues.<br>5. Preserve the tissue in one vial of preservative. (Make sure there is excess preservative; guard against diluting the preservative with too much water.)<br>6. Label the vial and put it on ice. Store on ice, in a freezer or refrigerator until the samples are shipped or analyzed (separate from food).<br>7. Clean tools and gloves, repeat for the next sample.  


=== Procedure B <br> ===
=== Procedure B  ===


(quicker alternative) - sampling oral arms or bell margin:<br>  
<br>(quicker alternative) - sampling oral arms or bell margin:<br>  


1. Collect medusae.<br>2. Flush the oral arms or bell margin with tapwater. Repeat several times to displace all debris.<br>3. Using clean forceps/scissors, cut a half-small-fingernail sized piece of tissue from the oral arm or bell margin. (It may be possible to do this simply by holding the tissue across an open vial of preservative and closing the lid.)<br>4. Preserve the tissue in one vial of preservative. (Make sure there is excess preservative; guard against diluting the preservative with too much water.)<br>5. Label the vial and put it on ice. Store on ice, in a freezer or refrigerator until the samples are shipped or analyzed (separate from food).<br>6. Clean tools and gloves, repeat for the next sample.  
1. Collect medusae, place it in a pail. Some scyphozoans are very fragile and so most care must be taken in handling them both before and after fixation to prevent damage. In general, this means keeping them suspended in liquid at all times and never handling them out of the water. Use a plastic tray or container to place the medusae.<br> <gallery widths=150px perrow=7>
Image:Handling1.jpg |Place the plastic bag below the specimen
Image:Handling2.jpg |Carefully catch the medusae with the plastic bag
Image:Handling3.jpg |Handle the jelly with  a plastic bag full of water
Image:Handling4.jpg |Place it in a plastic tray with sea water
</gallery>
<br>2. Flush the oral arms or bell margin with tapwater. Repeat several times to displace all debris.<br>3. Using clean forceps/scissors, cut a half-small-fingernail sized piece of tissue from the oral arm or bell margin. (It may be possible to do this simply by holding the tissue across an open vial of preservative and closing the lid.)<br>4. Preserve the tissue in one vial of preservative. (Make sure there is excess preservative; guard against diluting the preservative with too much water).  
<gallery widths=150px perrow=7>
Image:DNA1.jpg |With forceps hold a piece of oral arm and cut it with clean scissors or razor blades
Image:DNA2.jpg |Place the piece of tissue in a vial with 95% ethanol
</gallery>
<br>
<br>5. Label the vial and put it on ice. Store on ice, in a freezer or refrigerator until the samples are shipped or analyzed (separate from food).<br>6. Clean tools and gloves, repeat for the next sample.


=== Notes  ===
=== Notes  ===
Line 27: Line 39:
Both procedures A and B are designed to sample as much tissue and as little mesoglea (the 'jelly' of jellyfish) as possible. A third approach, not described above, is simply to preserve the whole animal, or a simple fraction thereof, if it has been cleared of potential contaminants and is small enough to fit easily into a vial with excess preservative (i.e. it is approximately &lt;1 cm bell diameter). The figure below indicates the tissues best suited to sampling. The same methods also can be used to preserve coronate jellyfish and stauromedusae for DNA analyses.<br>  
Both procedures A and B are designed to sample as much tissue and as little mesoglea (the 'jelly' of jellyfish) as possible. A third approach, not described above, is simply to preserve the whole animal, or a simple fraction thereof, if it has been cleared of potential contaminants and is small enough to fit easily into a vial with excess preservative (i.e. it is approximately &lt;1 cm bell diameter). The figure below indicates the tissues best suited to sampling. The same methods also can be used to preserve coronate jellyfish and stauromedusae for DNA analyses.<br>  


=== [[Image:SampleTissues.jpg|border|left|Sample Tissues]]Safety information  ===
[[Image:SampleTissues.jpg|border|left|Sample Tissues]] <br>
<br><br><br><br><br><br><br><br><br><br><br>
 
<br><br><br>
=== Safety information  ===


The chemicals in the DMSO+NaCl preservative are quite benign, being mostly water and table salt (see above). However, this information accompanies the two main chemicals.<br>1. DMSO (liquid, 20% of preservative by volume). "Causes skin irritation. Causes digestive and respiratory irritation. May cause severe eye irritation and possibly injury. May be absorbed through the skin. For eye contact, flush with water for 15 minutes and get medical aid immediately. For skin contact, flush with water and get medical aid. If ingested, do not induce vomiting and get medical aid immediately. If inhaled, remove to fresh air and get medical aid immediately."<br>2. EDTA (powder, @ 0.25M in preservative). "May cause irritation. For eye contact, flush with water and get medical aid. For skin contact, get medical aid if irritation occurs or persists. If ingested, give 2-4 cupfuls of milk or water and get medical aid. If inhaled, get medical aid if cough or other symptoms appear."  
The chemicals in the DMSO+NaCl preservative are quite benign, being mostly water and table salt (see above). However, this information accompanies the two main chemicals.<br>1. DMSO (liquid, 20% of preservative by volume). "Causes skin irritation. Causes digestive and respiratory irritation. May cause severe eye irritation and possibly injury. May be absorbed through the skin. For eye contact, flush with water for 15 minutes and get medical aid immediately. For skin contact, flush with water and get medical aid. If ingested, do not induce vomiting and get medical aid immediately. If inhaled, remove to fresh air and get medical aid immediately."<br>2. EDTA (powder, @ 0.25M in preservative). "May cause irritation. For eye contact, flush with water and get medical aid. For skin contact, get medical aid if irritation occurs or persists. If ingested, give 2-4 cupfuls of milk or water and get medical aid. If inhaled, get medical aid if cough or other symptoms appear."  
Line 35: Line 51:
Jellyfish stings can be at best uncomfortable and at worst lethal. Jellyfish must be handled with the utmost care, and protective clothing and gloves worn at all times. If you have any doubts, do not touch them. Ask for expert advice.  
Jellyfish stings can be at best uncomfortable and at worst lethal. Jellyfish must be handled with the utmost care, and protective clothing and gloves worn at all times. If you have any doubts, do not touch them. Ask for expert advice.  


<br>  
<br>


= DNA purification  =
= DNA purification  =
Line 41: Line 57:
= DNA amplification  =
= DNA amplification  =


= Preservation of medusae for morphological analysis  =
= Preservation of Medusae&nbsp;  =
 
Scyphozoans are typically preserved for morphological analyses in a solution of 4% formalin in seawater with the appropriate label (i.e. 4 parts formalin [37% w/v] and 96 parts seawater). Place the jellyfish in plastic container with a label (waterproof paper) and pour formalin until the organism is cover completely.[[Image:Morph1.jpg|thumb|center|Pour formalin until cover the medusae]]
 
If you are using a plastic bag, place the organisms in a bag, fill it with formalin, twist the bag, and use a rubber band to wrap the plastic bag. When is tight enough, fold the tip of the plastic bag and with the last part of the rubber band secure the folded part of the bag. Excess 4% formalin solution is used, and it can be renewed after two weeks to ensure successful fixation. <gallery widths="150px" perrow="4">
Image:Morph2.jpg | Place the organisms in a bag
Image:Morph3.jpg | Fill it with formalin
Image:Morph4.jpg | Twist the bag
Image:Morph5.jpg | Keep twisting the Bag
Image:Morph6.jpg | Hold the twisted part of the bag
Image:Morph7.jpg | Make a loop with the rubber band and hold the twisted part of the bag
Image:Morph8.jpg | Wrap the twisted part with the rubber band
Image:Morph9.jpg | Fold the tip of the bag and tight it with the rubber band
 
</gallery>
 
<br>
 
'''<br>'''
 
'''WARNING''' Formalin is highly toxic and should not be used without adequate protection, including overalls, gloves, and eye-glasses in a well ventilated space e.g. fume cupboard. Please consult the Materials Safety Data Sheet (MSDS) prior to use.<br> <br>


= Photography  =
= Photography  =


= FREE DNA Sequencing<br>  =
Good photographs are essential in two contexts. Good photographs of live animals in the ocean or in aquaria provide information on natural colour and shape. Good photographs of particular parts of jellyfish are important in species identification. Links to sites providing information on both these aspects are below.


Identify and sequence any scyphozoan for free! If you find a jellyfish and would like to know what it is and about it's DNA, then send pictures and a sample to us! We will identify the animals to the best of our ability as well as sequence molecular markers including "genetic barcodes" from the mitochondrial (16S rDNA, cytochrome c oxidase subunit I) and nuclear (18S, 28S, and other markers in the future) genomes, then send the information to you. All you need to do is follow the simple instructions below ...
== '''Photographing live medusae'''  ==


=== Photograph the jellyfish  ===
*See http://www.jellieszone.com/photography.htm Jellies Zone for tips on jelly photography.


=== Preserve the DNA ===
== '''Photographing particular parts of jellyfish to identify species''' ==


=== Preserve the remainder of the specimen for morphological analysis (optional, but highly preferred)  ===
In preparation. Please check back in a few weeks.<br>


=== Provide information about the collection ===
=== Materials and Method&nbsp; ===
[[Image:Materials.jpg|thumb|right|The picture only shows some of the materials being use. ]]


=== Conditions<br>  ===
*Tank (Black Background)
*RGB's
*Calipers
*Food Die (Purple, Blue, or Dark Green)
*Forceps
*Teasing Needles
*Scale Toothpick
*Hangers
*Insulin Syringes&nbsp;
*Ruler
*Measuring Tape&nbsp;
*Black Fabrics to use as Backgrounds&nbsp;
*Fluorescent Light Source&nbsp;
*Acrylic Table&nbsp;
*Photography Lighting Set&nbsp;


While we will endeavor to provide sequence data to you in a timely manner, turnaround will depend upon resources at the time. We expect that samples will be processed in less than one month in only exceptional circumstances. A more realistic expectation is 2-6 months, but sometimes longer as laboratory facilities may change from time to time. As resources are established and subsequently increased we hope to provide a more efficient service. Depending on your needs, arrangements can be made on a case by case basis. Please contact us if you have any questions.
<br>


We will attempt to sequence all species submitted, but success cannot be guaranteed. Our ability to generate sequence data will depend on the quality of the sample and whether existing techniques work for that species. If techniques don't work initially, we will attempt to modify them appropriately, but this will take time and sometimes may not be successful if resources (e.g. samples, time) are limited. Also, due to financial restrictions, we will only be able to sequence one or two jellyfish per species per location or region. If you would like to know whether we will sequence your samples before you send them, please contact us here. It may be possible to arrange a subset of analysis.
=== Procedure&nbsp;  ===


Submission of samples implicitly gives us the right to use the sequences, including, but not limited to, publication on this site and in the scientific literature. Our intention is to advance knowledge of the scyphozoans as broadly as possible. If this might conflict with your immediate interests, please do not hesitate to discuss the matter with us. We welcome the opportunity to collaborate with anyone interested in these animals and may forgo this condition in the interests of progress. All contributors to all studies will be acknowledged.<br>
=== Morphological Matrix&nbsp;  ===


=== Shipping<br> ===
[http://scyphozoan.ucmercedlibrary.info/wiki/Morphological_Matrix More Information]<br>


Please send all samples through airmail at room temperature to:<br>
=== Semaeostomeae  ===


<br>'''Dr. Michael Dawson<br>School of Natural Sciences<br>University of California at Merced<br>5200 North Lake Road<br>Merced, CA 95340 USA'''<br><br>
*[[Methods/Cyaneidae|Cyaneidae]]
*[[Methods/Ulmaridae|Ulmaridae]]
*[[Methods/Pelagiidae|Pelagiidae]]


See [[Shipping information and details]] for more information.<br>  
<br>  


<br>
=== Rhizostomeae  ===
 
*[[Methods/Cassiopeidae|Cassiopeidae]]
*[[Methods/Catostylidae|Catostylidae]]
*[[Methods/Cepheidae|Cepheidae]]
*[[Methods/Stomolophidae|Stomolophidae]]
*[[Methods/Mastigiidae|Mastigiidae]]
 
= Shipping information and details  =
 
[http://scyphozoan.ucmercedlibrary.info/wiki/Shipping_information_and_details <span style="text-decoration: underline;">For details on shipping</span>]<br>
 
[[Category:Identification]]

Latest revision as of 20:49, 31 August 2014

Preservation of DNA

(From: Dawson et al. 1998)

Equipment


1. Sterile syringes, forceps, dissecting scissors, or razor blades
2. A way of cleaning the sampling tools if they are not disposable (e.g. flaming metal objects after dipping in ethanol, or a good rinse and wipe dry)
3. Vials containing 1-2 ml of preservative (DMSO+NaCl or ethanol [70% to 95%; >90% preferred]; will be provided upon request).
4. Chest of ice (in the field); ice, refrigerator, or freezer (at lab/home, separate from food).
5. Protective gloves (latex, rubber).
6. Waterproof paper.
7. Plastic bags and/or jars.
8. Plastic tray or container.

Procedure A


Sampling gut or gonad:
1. Collect medusae.
2. Starve the medusae for as long as possible.
3. Using a clean syringe, flush the guts with tapwater. Repeat several times to displace any debris from the guts.
4. Using the same syringe (or other tool), suck up (tear or cut) about 0.1-0.2 ml of gastric and/or gonadal tissues.
5. Preserve the tissue in one vial of preservative. (Make sure there is excess preservative; guard against diluting the preservative with too much water.)
6. Label the vial and put it on ice. Store on ice, in a freezer or refrigerator until the samples are shipped or analyzed (separate from food).
7. Clean tools and gloves, repeat for the next sample.

Procedure B


(quicker alternative) - sampling oral arms or bell margin:

1. Collect medusae, place it in a pail. Some scyphozoans are very fragile and so most care must be taken in handling them both before and after fixation to prevent damage. In general, this means keeping them suspended in liquid at all times and never handling them out of the water. Use a plastic tray or container to place the medusae.


2. Flush the oral arms or bell margin with tapwater. Repeat several times to displace all debris.
3. Using clean forceps/scissors, cut a half-small-fingernail sized piece of tissue from the oral arm or bell margin. (It may be possible to do this simply by holding the tissue across an open vial of preservative and closing the lid.)
4. Preserve the tissue in one vial of preservative. (Make sure there is excess preservative; guard against diluting the preservative with too much water).



5. Label the vial and put it on ice. Store on ice, in a freezer or refrigerator until the samples are shipped or analyzed (separate from food).
6. Clean tools and gloves, repeat for the next sample.

Notes

DMSO+NaCl solution is 20% DMSO, 0.25M disodium-EDTA, and NaCl to saturation, pH 7.5 (Seutin et al. 1991); the pH of this solution must be >8 for the EDTA to dissolve, and warming promotes dissolution of NaCl. Sterilized by autoclaving prior to use.

100% ethanol is diluted to 80% (or greater) using purified drinking water (tapwater generally will suffice).

An important concern when sampling is to avoid contaminating the sample with tissues from other species (e.g. food) or with tissues from other individuals (see steps 2, 3, 7 in procedure A; steps 2, 3, 6 in procedure B).

Both procedures A and B are designed to sample as much tissue and as little mesoglea (the 'jelly' of jellyfish) as possible. A third approach, not described above, is simply to preserve the whole animal, or a simple fraction thereof, if it has been cleared of potential contaminants and is small enough to fit easily into a vial with excess preservative (i.e. it is approximately <1 cm bell diameter). The figure below indicates the tissues best suited to sampling. The same methods also can be used to preserve coronate jellyfish and stauromedusae for DNA analyses.

Sample Tissues
















Safety information

The chemicals in the DMSO+NaCl preservative are quite benign, being mostly water and table salt (see above). However, this information accompanies the two main chemicals.
1. DMSO (liquid, 20% of preservative by volume). "Causes skin irritation. Causes digestive and respiratory irritation. May cause severe eye irritation and possibly injury. May be absorbed through the skin. For eye contact, flush with water for 15 minutes and get medical aid immediately. For skin contact, flush with water and get medical aid. If ingested, do not induce vomiting and get medical aid immediately. If inhaled, remove to fresh air and get medical aid immediately."
2. EDTA (powder, @ 0.25M in preservative). "May cause irritation. For eye contact, flush with water and get medical aid. For skin contact, get medical aid if irritation occurs or persists. If ingested, give 2-4 cupfuls of milk or water and get medical aid. If inhaled, get medical aid if cough or other symptoms appear."

Ethanol is highly flammable. It should be kept away from naked flame and sources of heat at all times. It should not be transported except in small quantities packaged appropriately (check protocols for transporting hazardous substances).

Jellyfish stings can be at best uncomfortable and at worst lethal. Jellyfish must be handled with the utmost care, and protective clothing and gloves worn at all times. If you have any doubts, do not touch them. Ask for expert advice.


DNA purification

DNA amplification

Preservation of Medusae 

Scyphozoans are typically preserved for morphological analyses in a solution of 4% formalin in seawater with the appropriate label (i.e. 4 parts formalin [37% w/v] and 96 parts seawater). Place the jellyfish in plastic container with a label (waterproof paper) and pour formalin until the organism is cover completely.

Pour formalin until cover the medusae

If you are using a plastic bag, place the organisms in a bag, fill it with formalin, twist the bag, and use a rubber band to wrap the plastic bag. When is tight enough, fold the tip of the plastic bag and with the last part of the rubber band secure the folded part of the bag. Excess 4% formalin solution is used, and it can be renewed after two weeks to ensure successful fixation.



WARNING Formalin is highly toxic and should not be used without adequate protection, including overalls, gloves, and eye-glasses in a well ventilated space e.g. fume cupboard. Please consult the Materials Safety Data Sheet (MSDS) prior to use.

Photography

Good photographs are essential in two contexts. Good photographs of live animals in the ocean or in aquaria provide information on natural colour and shape. Good photographs of particular parts of jellyfish are important in species identification. Links to sites providing information on both these aspects are below.

Photographing live medusae

Photographing particular parts of jellyfish to identify species

In preparation. Please check back in a few weeks.

Materials and Method 

The picture only shows some of the materials being use.
  • Tank (Black Background)
  • RGB's
  • Calipers
  • Food Die (Purple, Blue, or Dark Green)
  • Forceps
  • Teasing Needles
  • Scale Toothpick
  • Hangers
  • Insulin Syringes 
  • Ruler
  • Measuring Tape 
  • Black Fabrics to use as Backgrounds 
  • Fluorescent Light Source 
  • Acrylic Table 
  • Photography Lighting Set 


Procedure 

Morphological Matrix 

More Information

Semaeostomeae


Rhizostomeae

Shipping information and details

For details on shipping