Beruflich Dokumente
Kultur Dokumente
Research Project:
DEVELOPMENT OF
Advanced Search DETECTION Project Team
TECHNOLOGIES FOR
TOXINS AND THEIR Brandon, David
VALIDATION IN FOOD Stanker, Larry
MATRICES
Location: Foodborne Carter, John - Mark
Contaminants Research Cheng, Luisa Wai Wai
Title: Development and Partial Hernlem, Bradley - Brad
Programs and Characterization of High-affinity
Projects Monoclonal Antibodies for Rasooly, Reuven
Subjects of Botulinum Toxin Type A and He, Xiaohua
Investigation their use in Analysis of Milk by
Sandwich ELISA
Authors
Stanker, Larry Publications
Merrill, Paul
Publications
Scotcher, Miles
Cheng, Luisa Wai Wai
Submitted to: Journal of
Immunological Methods Related National Programs
Publication Type: Peer
Reviewed Journal Food Safety, (animal and
Publication Acceptance Date: plant products) (108)
March 4, 2008
Publication Date: April 9, 2008
ProSci can help you develop custom monoclonal antibodies and we understand
researchers have varying needs for levels of involvement, depending on the target. We
have developed monoclonal antibody development packages for different levels of
involvement in the project, from researcher screening (you screen positive wells
following fusion for clones of interest) to ProSci sending western blot and
immunocytochemistry positive final clones. We offer custom monoclonal antibody
development packages for both protein and peptide antigens. Our screening options
include:
• ProSci sends final clones, guaranteed ELISA positive. (no additional charge)
• Researcher screening of positive wells, following fusion. (starting at $500)
• Western Blot screening: ProSci screening of positives during Phase 2 (Fusion)
and Phase 3 (Sub-cloning) for Western Blot positive clones.
o Protein antigens: guarantee of up to 3 western blot positive clones.
($2200-$2600)
o Peptide antigens: cannot guarantee reactivity, but >70% success rate;
see Terms & Conditions for more details. ($2200-$2600)
• ICC screening: ProSci screening of positives during Phase 2 (Fusion) and
Phase 3 (Sub-cloning) for immunocytochemistry positive clones
o Protein antigens: guarantee of up to 3 immunocytochemistry positive
clones. ($2600)
o Peptide antigens: cannot guarantee reactivity, but >70% success rate;
see Terms & Conditions for more details. ($2600)
• Western blot & immunocytochemistry screening: ProSci screening of positives
during Phase 2 (Fusion) and Phase 3 (Sub-cloning for Western Blot AND
immunocytochemistry positive clones. ($4200)
ProSci’s fusion success rate for custom monoclonal antibody developement is greater
than 95%, using techniques developed in-house. All work is performed by skilled
technicians on premises in our San Diego, California laboratories. Your custom
monoclonal antibody production project, and can be scaled up to almost any
magnitude. We can screen against multiple antigens (additional charges apply) to
develop the specific clone you need. ProSci has repeatedly proven our abilities to
produce hybridomas against difficult targets.
Fusion Partners (protein antigens): If you are submitting a protein antigen for
custom monoclonal antibody developement, we highly recommend cleaving large
fusion partners such as GST tags. These tags tend to be highly immunogenic, and if
they are not removed prior to immunization, a dual screening process must be
performed. This ensures positive responses are to the protein, not the fusion partner.
To do this we perform dual ELISA screening, screening for high ELISA titers against
the protein and low ELISA titers against the fusion partner. This additional service is
available at $2400 per additional screening.
The identification of genetic biomarkers and pathways has revolutionized the process
of drug discovery and created a flurry of novel therapeutic targets and methods. In
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of a therapy through clinical trials and beyond. MBS has partnered with top
pharmaceutical companies, using 19 years of antibody development experience and
proprietary protocols, to provide the best possible antibodies to monitor their
therapeutic applications.
Spleen cells from the selected animal are fused with myeloma cell line to develop a
hybridoma that secretes a specific antibody. Once your mice or rats are ready for
fusion per ELISA screening results, a fusion is performed. The fusion is plated and
screened. The primary screening is a direct ELISA against your antigen to capture all
positive fusion products. The positive fusion products are scaled up and screened
again. The secondary screening differentiates between IgG and IgM clones, and
verifies that the selected positive fusion products are still producing antibody prior to
cryopreservation. You will choose the number of fusion wells for scale-up. Not all
wells that are scaled up will survive or continue to produce specific antibody. The
supernatants of the positives are shipped to you for further testing. At this point, MBS
is able to offer small amounts of purified antibody from the fusion products through a
process called MultiPure. Learn more about MultiPure
Phase 4: Subcloning
For cell lines developed in Balb/c mice, we typically use 10 Balb/c mice to produce
Ascites. If your cell line was developed in rats, we will produce a Spinner Flask
production or run a nude mice ascites production. The ascites or spinner flask
production can be purified by Protein A or Protein G when the antibody is an IgG.
The final monoclonal antibody is shipped to you within 7-8 weeks of selecting a
subclone.
Contact us today to learn more about our Monoclonal Antibody and Hybridoma
Development Program.
Protocol On-line
http://www.protocol-online.org/prot/Immunology/
Immunochemistry Protocols
Pharma-Lexicon
Search Medical abbreviation, Pharmaceutical Companies and Associations. Refer to
existing MBS site www.mainebiotechnology.com for more info:
13. Inject 2-10x106 recloned hybridoma cells into BALB/c mice which
had received an i.p injection of 0.3 ml of pristane 7 days previously.
Collect ascites 7-21 days latter.
REAGENTS
Media:
Hy-HAT:
to make 100 ml
RPMI-1640 - 77 ml
NCTC-135 - 10 ml
FCS (hyclone) - 10 ml
Hy-HT:
HyM-(HT or HAT):
HT concentrate (100x):
Fusion reagent:
PEG-4000 - 10 g (melted)
DMSO - 1 ml
Filter sterilize with 0.45 micron filter. Store at room temperature. Stable for several
months.
Hemolytic reagent:
NH4Cl - 0.83 g
Adjust pH to 7.2 with HCl. Dissolve in 100 ml d. water. Filter sterilize with 0.2
micron filter. Store at 40 C. Stable for several months.
Ethanol 70%
Two 60 mm petri dishes, one with 3 ml and the other containing 10 ml of M-10
medium.
One tissue sieve (100 squares/inch) and pestle in a 100 mm petri dish. The sieve
screen and pestle face should be wetted with M-10 and the petri dish contain 15 ml of
this medium.
Combine cell pellets and resuspend cells in 5 ml of ice cold hemolytic reagent.
Incubate at room temperature for 10 minutes and add 5 ml of ice cold M-10 medium.
Immediately centrifuge at 1,000 rpm for 5 minutes . The cell pellet should be
erythrocyte-free and contain approximately 100 x 106 cells. If the cell pellet has any
red coloration indicating the presence of unlysed erythrocytes, the cells should be
suspended in additional 10 ml of ice cold M-10 medium and recentrifuged. When the
spleen cell pellet is free of red blood cells, combine with 100 x 106 NS-1 BALB/c
myeloma cells by resuspending the cells in 15 ml of M-0 medium at room
temperature. Centrifuge at 1,000 rpm for 5 minutes, aspirate of the supernatant and
resuspend cell pellet for a second wash in M-0 medium. Centrifuge as above and
aspirate off all the supernatant to give a "dry" cell pellet.
CELL FUSION
Set a timer for 6 minutes. Quickly resuspend the cells in 0.5 ml of 50% PEG-4000
and start the timer. After 2 minutes, add 0.5 ml of M-0 medium and carefully mix.
After each additional minute, add another 0.5 ml of M-0 until the end of 6 minute
period. At this time, finish filling the test tube with M-0. Carefully invert to mix thus
diluting the PEG.
Centrifuge at 750 rpm for 3 minutes and aspirate off the supernatant. Carefully add 10
ml of HAT medium at a rate sufficient to dislodge the pellet without dispersing the
cells. Allow the fused cells to "rest" for 10 minutes then draw the cell pellet into a
pipet and expel with just enough force to disperse the cells. Pipet the cells into a
75cm² tissue culture flask in a total of 50 to 60 ml of HAT medium. Incubate in a 5%
CO2 incubator at 370 C for 2 days, then distribute the cells evenly into eight 96-well
microtiter plates. The plates have had either 3,000-6,000 peritoneal macrophages
added per well in 60-100 µl of HAT medium or the HAT medium should be
supplemented with 50 µg/ml of LPs and 20 µg/ml of dextran sulfate. If the mouse's
spleen cells respond well to these mitogens, the hybridomas will probably grow faster
and produce more clones than with peritoneal macrophages. A drawback to using
mitogen stimulation is that some hybridomas may develop a nutritional requirement
for LPs or dextran sulfate.
Cultures should be feed with one drop per well ( approx. 60 µl ) of fresh medium
every 3-5 days. When a well is full, one-half of the volume of the well should be
removed by aspiration using a sterile pasteur pipet and a drop of fresh medium added.
RECLONING
When a microtiter well tests positive for the antibody of interest it is important to
reclone as soon as possible to avoid the potential loss of the positive clone due to
overgrowth by non-secreting cells. Recloning can be accomplished by either growing
the hybridoma in soft agar or by a limiting dilution technique. I have personally better
success with the latter method.
Limiting dilution recloning first requires an accurate cell count of the viable
hybridoma cells suspended in the medium of the microtiter well in which the cells are
growing. Next the cells are diluted so that when one drop of cell suspension is placed
in each well of a 96-well microtiter plate, the average number of hybridoma cells will
be 0.5, 1 and 3 cells per well. At least one plate ( 96 wells ) should be prepared for
each dilution. If there is growth in 5 wells or less, the odds are greater than 95 % that
the clones are monoclonal. If less than 80 % of the clones tested are positive, the
hybridoma should be recloned a second time. When the dilutions listed above give to
little or to much growth an appropriate adjustment to either a higher or lower dilution
is required. The cloning efficiency of hybridomas can be greatly enhanced by the
addition of 3,000-6,000 peritoneal macrophages per well or by including LPs and
dextran sulfate in the cloning medium.
The fastest growing clones producing the most antibody are selected for clonal
expansion. Several ampules of each clone chosen for expansion should be prepared
for storage in liquid nitrogen using a standard cell freezing technique.
Antibody can be purified and concentrated from the hybridoma conditioned growth
medium or high titer ascitic fluid can be prepared.
The NS-1 myeloma cell line is BALB/c origin so if the spleen cells are from any other
mouse strain then ascites should be produced in the F1 cross between BALB/c and the
other mouse strain. In all of the fusions I have prepared the spleen cells were from
BALB/c mice and therefore this mouse strain was used to produce ascitic fluid.
The mice are first primed with an intraperitoneal injection of 0.3 to 0.5 ml of pristane.
Pristane is a C14 branched oily hydrocarbon which induces, in primed mice, an oil-
granuloma. This environment is optimal for acceptance and growth of hybridomas
and allows the antibody titer in ascitic fluid to reach levels 100 to 10,000 times greater
than can be achieved in tissue culture medium.
Seven days after the mice are primed, one to ten million hybridoma cells are washed
with sterile PBS and injected into each mouse. Seven to twenty one days latter the
ascites is collected by inserting a 1 1/2" x 19 GA needle into the swollen peritoneum
in the inguinal area and parallel to the spine. The mouse is positioned with the needle
hub over a test tube and the ascitic fluid is collected by gravity flow. 1-8 ml of fluid
can be obtained from each mouse.
Now the ascitic fluids allowed to clot and the cells and fibrin are removed by
centrifugation. Heat inactivate at 560 C for 20-25 minutes. Next, centrifuge at high
speed to clarify and aliquot in 1 ml to vials and store in -700 C freezer.
The mouse is prepared as for splenectomy except the abdominal musculature is left
intact. A 5 cc. glass syringe is fitted with a 1 1/2" x 18 GA needle and filled with 5 ml
of refrigerator cold (4-80 C) 0.34 M sucrose ( dissolved in distilled water and filter
sterilized through a 0.2 micron filter). A medial and enteral part of the abdominal
musculature is held away from visceral organs with a sterile forceps to form a space
for 3 ml of the sucrose solution to be injected. The needle is withdrawn and the
abdomen massaged for about 15 seconds to insure maximum suspension of resident
macrophages.
The abdominal musculature is again held with the forceps and the needle reinserted.
The remaining 2 ml of sucrose in the syringe is forcefully injected into the abdominal
cavity thus mixing with the cell suspension. This cell mix is then withdrawn into the
syringe, care being taken not to puncture any organs with the needle while removing
as much of the cell suspension as possible. The cell suspension is transferred into a
sterile Teflon tube, enumerated, then capped and centrifuged at 1,200 rpm in a IEC
PR-6000 centrifuge for 7 minutes. A tube of Teflon is used as macrophages will
tenaciously adhere to glass and most plastic, but will not adhere to Teflon.
The cells form a lose pellet so care must be exercised when aspirating the supernatant
not to disturb the pellet. 0.5 to 0.7 ml of sucrose solution can remain with the cells
with no adverse effect on the hybridoma culture. 80-90 % of the resident peritoneal
cells should be macrophages, while the majority of remaining cells are lymphocytes.
2-4 million cells should be recovered per mouse. The cells are now ready to be diluted
in Hy-HAT medium and used as hybridoma feeder cells.
Reagents:
1-3 x 10 8-9 immune spleen cells
1-6 x10 7-8 myeloma cells in log phase of growth
Complete Media No Sera (CMNS) for washing of the myeloma and spleen cells.
Hybridoma medium CM - HAT {Cell Mab (BD), 10% FBS (or HS) ; 5% Origen HCF
(hybridoma cloning factor) containing 4mM L-glutamine and antibiotics} to be used
for plating hybridomas after the fusion.
Thawed inactivated and pre-filtered commercial Fetal Bovine serum (FBS) or Horse
Serum (HS) stored in the refrigerator at 40C. Must be pretested for myeloma growth
from single cells.
Cell Mab Media, Quantum Yield from BD is stored in the refrigerator at 40C in the
dark. Myeloma growth media is Cell Mab Media with added L-gln to 2 mM and
antibiotic/antimycotic solution to 1% and is called CMNS. Do not add antibiotics to
media when growing myelomas for stock, only for pre-fusion growth. Indicate
presence or absence of each reagent on the bottle label. Do not adjust the pH as it
contains HEPES biological buffer already.
1 bottle of PEG 1500 in Hepes (Roche) (use fresh bottle that has never been opened)
Myeloma Media is CM which has 10% FBS (or HS) and 8-Aza (1 X) stored in the
refrigerator at 40c.
Clonal cell medium D (Stemcell, Vancouver) contains HAT and methyl cellulose for
semi-solid direct cloning from the fusion. This comes in 90 ml bottles with a CoA and
must be "melted at 37Oc in a waterbath in the morning of the day of the fusion.
Loosen the cap and leave in CO2 incubator to sufficiently gas the medium D and
bring the pH down.
Origen HCF can be obtained directly from Igen and is a cell supernatant produced
from a macrophage-like cell-line. It can be thawed and aliqouted to 15 ml tubes at 5
ml per tube and stored frozen at -200C. Positive Hybridomas are fed HCF through the
first subcloning and are gradually weaned. It is not necessary to continue to
supplement unless you have a particularly difficult hybridoma clone. This and other
additives have been shown to be more effective in promoting new hybridoma growth
than conventional feeder layers.
Procedure At least one week prior to expected fusion date thaw a fresh vial of
myeloma cells. It is advisable to keep several flasks at different densities so that you
can choose the best one on the day of the fusion. We generally try to use a flask that is
actively dividing and at a cell density of 3-6x105 cells/ml. Do not let them overgrow
or they will enter a decline phase.
Two to five days before the scheduled fusion give a final injection of ~5ug of antigen
in PBS i.p. or intravenously in tail vein of the mouse (with high titer already
determined).
1. Spin down myelomas and wash with 30 ml serum free media (CMNS has
glutamine). Use tabletop centrifuge at 850 rpm for 12 minutes. Perform viable cell
count with trypan blue exclusion principle, and wash cells with 30 ml of RPMI-
CMNS. Spin down as above, resuspend in CMNS and disperse. Leave at 37°C until
spleens are retrieved.
Test aminopterin sensitivity. Keep 1 million myeloma cells for control plate and
transfer into a 15ml conical. To do so, add 15 ml of HAT media to the million
myeloma cells and plate out 2 drops/well on a 96 well plate.
2. Remove spleen from mouse in the biohazard facility. Euthanise the mice and
submerge it in 70% ETOH. Let the mouse air dry on its right side on a paper towel.
Remove spleen using sterile instruments and carefully put into labeled 10 ml of
RPMI-CM with antibiotics and 20% FCS for transport back to the lab. Dispose of
mouse and leave facility.
3. Place spleen into sterile petri dishes. Add 10 ml of RP-I-CMNS and perfuse the
cells out of the spleen. Poke the spleen 8-10 times with an 18 ga needle (hold with
sterile forceps). Use a 21 ga on a 3 ml syringe to draw up some RPMI. Inject the
RPMI slowly into the spleen about 50-100 times until nearly all the cells are washed
out. Discard the spleens into the biohazards bag.
4. Collect and transfer the spleen cells to a new 50 ml conical tube. Rinse out the dish
2X with 10 ml of RPMI-CMNS and pool with the first 10 ml (the use of perfusion
removes the production of large debris seen with grinding, and obviates the need to let
the debris settle). Spin down at 900 rpm for 12 minutes. Discard the supernatant to
bleach container. Wash the cells with another 30 ml RPMI-CMNS. Remove a small
sample and count the viable cell/ml and spin again as above. Combine the cells at a
ratio of 5:1 (spleen cells: myeloma cells) and never 1X10 myeloma cells.
5. Wash both the myeloma and spleen cells 2 more times with 30 ml of RPMI-CMNS.
Spin at 800 rpm for 12 minutes.
7. Aspirate all fluid into bleach vessel. Break up pellet by gently tapping on the flow
hood surface. Add 1 ml of BMB REG1500 (prewarmed to 37°C) dropwise with 1 cc
needle over 1 minute. Swirl and tap the conical gently while adding the PEG to
resuspend the cells.
8. Add 1 ml of RPMI-CMNS to the PEG cells gently over 1 minute while swirling (to
dilute the PEG).
10. Incubate the cells in the 37°C waterbath for 10 minutes. Centrifuge the cells at
700 rpm for 10 minutes (the membranes are still very weak).
13. Gently dilute cells in 5 ml of Complete media and transfer into 95 ml of Clonacell
Medium D (HAT) media (with 5 ml of HCF) and plate out 10 ml per small petri plate.
14. Dilute about 1000 P3X63 Ag8.653 myeloma cells into 1 ml of mediu D and
transfer into a single well of a 24 well plate. This is the myeloma/HAT control. P
15. Place plates in incubator two plates inside of a large petri plate, with an additional
petri plate full of dH20 without a lid for humidity. Leave for 10-18 days under 5%
CO2 overlay at 37 degrees.
15. Pick clones from semisolid agarose into 96 well plates containing 150-200 ul of
CM- HT. Screen sups 4 days later in ELISA. Move positive clones up to 24 well
plates.
16. Heavy growth will require changing of the media at day 8 (+/- 150 ml). Should
see macroscopic colonies at this time.
At this time can decrease the HCF to 0.5% (gradually- 2%, then 1%, then 0.5%) in the
cloning plates.
17. Isotype via supernatants and grow up for ascites/ large flask production and
further freeze down. Troubleshooting
I strongly reccommend to use Southern Biotech Goat anti-Mouse Ig (H+L)HRP
Chains for screening supernatants. We have screened and developed Mabs to various
antigens and have surprisingly found out that using some secondary reagents from
several other major companies can result in weak or no reactivity.
2) Lane, R.D. A short duration polyethylene glycol fusion technique for increasing
production of monoclonal antibody-secreting hybridomas. 1985. J. Immunol. Meth.
81:223-228.
5) Zhong, G., Berry, J.D., and Choukri, S. (1996) Mapping epitopes of Chlamydia
trachomatis neutralizing monoclonal antibodies using phage random peptide libraries.
J. Indust. Microbiol. Biotech. 19, 71-76.
6) Berry, J.D. , Licea, A., Popkov, M., Cortez, X., Fuller, R., Elia, M., Kerwin, L., and
C.F. Barbas III. (2003) Rapid monoclonal antibody generation via dendritic cell
targeting in vivo. Hybridoma and Hybridomics 22 (1), 23-31.
Monoclonal Antibody
Production
Mouse Immunization
Order 6 six week old Balb/C mice and let the ARC know they are coming.
Have your antigen ready for when they arrive. Once they get there earmark
the mice and perform a pre-bleed on them to be used as an ELISA control
for monitoring the titer and screening of the hybridomas:
Bleeding Mice
1. Place the mouse in a mouse restrainer.
2. Sterilize the tail with 70% ethanol.
3. With a razor blade, nip off the last 2 mm of the tip of the tail.
4. Using a milking motion, pull blood down and let drip off the end of
the tail until you have collected ~200 µL. (You may have to pre-bleed
twice, with a week or so between bleeds).
5. Take the collected blood and place at 37 °C for 30 min. to remove
complement.
6. Place blood at 4 °C overnight to clot.
7. Centrifuge samples at 10,000g 10 min.
8. Pipet off the serum supernatant. Store at -20 °C. This is your pre-
bleed control.
Hybridoma Fusion
For one fusion you will need:
Immunological Techniques
Introduction
Monoclonal antibodies are great! Why? Specificity! Each one recognizes only one site of the antigen
structure. Why else? Immortality! Mass cultures can be generated from a single clone.
Mice are small! They require less antigen than a rabbit to get an antibody reaction. The antigen travels
through the circulation system. Blood is channeled through the spleen where B lymphocyte cells
recognize the foreign bodies and produce antibodies.
Spleen cells, however, cannot survive alone in tissue culture media. Myeloma cells can! Why not fuse
them?
We can select for fused cells by using a HAT (hypoxanthine, aminopterin, thymidine) supplemented
media. The mutant myeloma cell line SP2/0 cannot survive in HAT media because it lacks HGPRT.
The aminopterin in the HAT supplement blocks DNA synthesis. The enzyme HGPRT can overcome
this block. Spleen cells do have HGPRT. Fuse the spleen and SP2/0 cells and you'll find survivors in
HAT tissue culture media.
Notes:
If you pour (you really should pipet) DON'T SPILL! Contamination occurs because
of spillage outside of bottles and tubes. Ethanol and flame when you're feeling
paranoid.
Use disPo products to avoid problems with detergent residue on washed glassware.
Supplies:
1cc syringe
Immunization
Coomassie stain for an hour & destain (10% acetic acid, 45% methanol) as quickly as possible, cutting
the bands as soon as they are discernible to limit the time that the gel is in acid. Rinse with PBSa & cut
out the bands. Protein can be stored with a small amount of PBSa in the -20 freezer.
Make first injection of protein at 1:1 ratio with Freund's Complete or TiterMax.
1. Homogenize protein with a small amount of PBSa so protein doesn't get too thick.
Keep protein cold while homogenizing.
2. If using Freund's, mix up dead bacteria in the bottle. Draw Freund's into a syringe
and force it out into a small beaker containing your protein sample. Mix the Freund's
and your protein until it takes on a white foamy consistency. You may have to change
needles and syringes because the Freund's reacts with the plastic.
e.g. To inject 6 mice with emlc and rmlc each, I ran one 12% gel, cut out the bands,
homogenized the protein and combined each protein sample with 450ul of Freund's.
This gave me a little over 600ul of each sample to inject.
notes:
• Your sample must be concentrated but not so thick that you cannot get it through a
1/2 inch, 25g needle.
Two weeks later, make second injection of protein with Freund's Incomplete Adjuvant or TiterMax.
Two weeks later, do a test bleed. If negative, do another boost with Freund's Incomplete Adjuvant or
TiterMax.
Five days before the fusion, do a final boost of protein without Freund's.
Test Bleeds
Apply grease to tail (an area of 3/4 inch, from base toward tip).
Use extremely sharp blades to make slice (EM blades). Be careful not to cut through the tail but make
cut large enough to draw about 2.5 heprinized capillary tubes.
Spin down the blood at max speed for 5 minutes in the microfuge.
Draw off and store sera at -20o until you can test on a blot at 1:100 or at 1:50.
WED/THURS
Thaw out a plate of SP2/0, split one to 3. (must split during weekend). Need 10-12 100mm plates in log phase
for fusion.
Thaw tube quickly in 37o bath. Put into falcoln tube with 10ml of warm media. Let sit for 5 min. Spin
down at low speed. Resuspend in 10 ml and spin. Resuspend in 30ml and put into 3 plates.
THURS
FRI
MON
TUES
Do Fusion!
Collect
2 x 10 ml petri dishes
disPo 10 ml pipets
5 ml Sodium pyruvate
5 ml L-glutamine
HAT(with syringe, pump 5ml DMEM into HAT bottle, add to DMEM)
Put into 5 x 50 ml conical tubes (to later be transferred to 5 flasks for feeder layer).
Dissection
WORK QUICKLY! (The slower you are, the more difficult it is to work with the animal. Also, you
don't want the media to cool.)
• Sacrifice the mouse. Ethanol until saturated. Pin the animal in place.
• Use one set of utensils to cut through the skin, pin back the flap. ETHANOL!
• Use third set to pull out the spleen, cutting away the connective tissue.
Wash Cells
• Put spleen in the dish with 10 ml of DMEM-. Quickly and carefully disperse spleen
cells with plunger of a 5 ml syringe against the screen.
• Leaving connective tissue on the grid, pipet up and down and put cells into a 15ml
conical tube. Let large chunks settle to the bottom of the tube for 2-3 min.
• Carefully, suck off supernatant with sterile pasteur pipet. Wash spleen cells again
with 10ml DMEM-.
• Suck off super. Resusp. in 5ml DMEM-, incubate for 10 min. in 37o bath. Pour 5x
50ml conicals of DMEM+ into tc flasks. Put 1ml of spleen cells in each flask.
• Incubate o/n in 6% CO2 37o chamber. Lay flasks on sides with caps loosened.
FUSION DAY
Collect
• All of the same supplies used for the feeder layer on previous day.
Filter sterilize leftover DMEM+ media from yesterday followed by feeder layer. The feeder layer is
more likely to clog the filter. (Make sure you have media in the container before turning on the vacuum otherwise you could
break the filter membrane).
Follow protocol used to dissect the mouse for the feeder layer.
It is important to minimize the time that the spleen cells are either not in the animal or not in the
incubator. For this reason and depending on how quickly you are able to dissect the mouse, you may
want to collect the SP2/0 cells first.
Spin down the cells. Wash cells 2x. Pellet for 10 min. at 170g.
resusp spleen cells, wash, pellet WHILE resusp one tube in 5ml, transfer to
resusp spleen cells in 10 ml, count, WHILE resusp SP2/0, wash, pellet
• Add 1.5 ml PEG over 1 min. under agitation-- THIS IS THE FUSION!!!
• Over the next min, add 1ml of warmed DMEM- while stirring.
Screening
Draw off 500ul & test on blot strips, incubate overnight. (Don't forget positive controls including
mouse antibody - use mouse polyclonal sera and a marker.)
Both should be positive. Continue to split positive plates and freeze down (in 10% DMSO) as back ups.
Triterate and dilute cells from the positive well into a 96 well plate at a dilution of 1 cell to ~3 wells.
We're going for the single clone!
Pass through dilution again until all wells are testing positive and you are convinced that you have a
monoclonal cell line.
Eventually, try and wean the cells from 10% FCS to 5% FCS, and from HAT to HT to unsupplemented
media.
Buffers:
start with the dibasic solution and titer with the monobasic until pH 7.0 is reached
3.75 g glycine
bring to 500 mL with water
Protocol
2. Put sample over column - 10 mL rabbit serum for IgG isolation or entire volume of
papain digestion - take gel samples. (Flow rate at 1mL/4 min)
3. Save pass through - in papain digest the pass through contains the Fab - take gel
samples.
6. Collect 0.5 mL fractions and neutralize solution with 1.0M Tris to pH 7.4 (use
indicator strips)- take gel samples. Spec fractions to find peak.
7. Wash with pH 3.0 buffer for 15 minutes and store in 20% ethanol.
9. Determine concentration using spec at absorbance of 280nm with A280 of 1.35 for
IgG or 1.5 for Fab.
1. Run SDS-PAGE curtain. (Use as much protein as possible without having so much
that you risk running bands together and contaminating the band of interest).
2. Place unstained gel in 0.5 M KCl for 10-15 seconds -- until bands begin to appear.
The bands will appear clear, while the rest of the gel will turn white as the SDS
precipitates. Remove the gel onto a glass plate and cut out band of interest as rapidly
as possible. If you wait too long, the bands will turn white as well.
3. Place gel strip(s) into 50 mM NaPO4, pH 6.5 with 0.1% SDS and rinse 3 times,
with gentle shaking, for 30 min. per rinse.
4. At third gel wash, begin activation of the APT paper. Do these steps in the cold
room on an ice bath. First, place an appropriately-sized piece (slightly larger than
gel) of APT paper in cold 1.2N HCl (100 ml) to which has been added 3 ml of
sodium nitrite (NaNO2). The NaNO2 is made in water at 10 mg/ml immediately
before use. Incubate paper on ice with occassional shaking for 15-30 min. The paper
should turn bright yellow. Activation is followed by two or more rapid ice water
washes and two rapid washes with 50 mM NaPO4 pH 6.5, taking 5 minutes for the
whole process. (When I originally did this, I used a protocol which called for 5 X 5
minute washes with ice cold water and a subsequent 10 min wash in cold 50 mM
NaPO4, pH 6.5. However, Bio-Rad emphasizes the necessity of short washes. Both
seemed to work for me.)
5. Immediately after activation, set up the transfer in the cold using 50 mM NaPO4,
pH 6.5 as transfer buffer. Transfer for 4 hours at 0.6 amps (Hoefer TE-52). The paper
should have turned an orangey (peach) color. Ususally where the gel was, the color is
lighter.
6. Block the DPT paper in the following buffer for 2 or more hours:
20 ml ethanolamine
20 ml 1 M Tris-HCl pH 9.0
_______________________
7. Rinse extensively in "Buffer 1" following the blocking step. Do at least 3 20-30
minute washes.
Buffer 1:
50 mM Tris-HCl, pH 7.5
5 mM EDTA
150 mM NaCl
8. To check transfer efficiency, cut a strip off one side of DPT paper to which protein
has been transferred and incubate with your (appropriately diluted) antibody
overnight. (Dilute the antibody in Buffer 1 containing 0.25% gelatin, or 1% BSA
[Sigma Fraction V]. I use BSA.) Carry through with normal protocol for
immunobloting, i.e. rinse (3 changes of buffer 1 or PBS) 30 min, incubate 2-4 hours
in peroxidase conjugated secondary antibody, rinse, develop in 0.05% 4 chloro-1-
napthol (made up as a 0.3% solution in methanol), 0.01% H2O2 in PBS. The reaction
seen on the DPT paper is usually not as distinct as that seen on nitrocellulose.
9. If you are waiting to check efficiency of transfer before using the DPT paper, just
store paper in Buffer 1 at 4o C until use.
a. cut paper into small squares (on a glass plate) with a clean razor blade.
d. the next morning, squirt out diluted antiserum (from which epitope specific
antibodies have presumably been removed) and draw about 10 ml of Buffer 1 into the
syringe. Shake rapidly and repeat for a total of 3 rinses (30 minutes each)
e. to elute specific antibodies, use 4 ml of 5 M NaI made up fresh in ice H2O. Draw
up into syringe and place on ice; agitate by rotation of the syringe on ice for 8
minutes
f. force the NaI solution (now containing eluted antibodies) into a tube (50 ml Falcon
type) containing 600 ll of Buffer 1/1% BSA. Force Buffer 1 through DPT paper
repeatedly, pooling all of these washes in the same 50 ml tube until a total of 40 to 50
mls is reached. (You may have to dilute even further if the intended use of the
antibody is for immunofluorescence. Concentrations of salt that are too high interfere
with fluorescence visualization).
g. To concentrate antibody:
Alternative #1.
11. Store DPT squares in the syringe in Buffer 1 at 4oC. I've never used azide but have used squares
repeatedly (up to 10-12 times) over a period of 6 months without any problems.
Immunoprecipitation
1. Harvest 5 x 106 - 4 x 107 cells/sample depending on how abundant your protein is.
Use 5 x 106 cells/sample to IP myosin, 4 x 107 cells/sample to IP dynein, for example.
Wash cells a couple of times in DB, and resuspend in 500 µ l DB/sample. Place on
ice.
2% NP40
10 mM EDTA
50 mM NaPPi
200 mM NaF
5 mM DTT
2 mM PMSF
2 mM ATP
40 mM Tris, pH 7.5
0.2% NP40
2 mM DTT
10 mM EDTA
2 mM PMSF
200 µ M TPCK
200 µ M TLCK
20 mM NaHSO3
50 mM NaPPi
200 mM NaF
2 mM ATP
200 mM KPO4
5. Collect cleared lysate. Use 1 ml lysate per IP sample. Add primary antibody:
For 396 myosin Ab, preincubate 25-30 µ l GammaBind or protein A-sepharose beads
with 1 ml of 396 supernatant for 4 hours to overnight. Wash beads as per steps 10-11
below and resuspend beads directly in 1 ml cleared lysate. Skip steps 6-7 and go
directly to step 8.
7. Add 25-30 ul protein A-sepharose slurry for rabbit and rat primary antibodies; add
25-30 ul GammaBind slurry for mouse primary antibodies.
10. Wash beads twice with 1 ml each time of 1X IP buffer with 1 mg/ml BSA (to
reduce background, adjust pH of IP buffer to 7.0 for washes). Spin down as above.
11. Wash beads twice with 1 ml each time of 1X IP buffer, pH 7.0 without BSA. Spin
down as above.
12. If desired, do a final wash in 1X IP buffer with 0.5M NaCl. This will further
reduce your background. HOWEVER, it will strip the dynein IC off the HC when
doing IPs with NW127 Ab!
13. Remove all traces of wash buffer, and resuspend beads in 20-30 µ l 2X SDS
sample buffer. Boil 5 minutes. Spin down beads, load super onto an SDS gel. IgG
heavy chain runs at 50 kd; IgG light chain runs at 22 kd.
notes: If you have a lot of background, it may help to preincubate the cleared lysate with beads
(without antibody!) for a couple of hours to adsorb out any non-specific binding. Spin down the beads,
recover the lysate, and add primary antibody. Proceed with step 5.
1/95, Trivinos
2. Ice-cold 2 x lysis buffer was then added to the cells suspension. (40 mM Tris-Cl
pH7.5, 0.2% NP40, 2mM DTT , 10 mM EDTA, 2 mM PMSF, 2 mM TAME, 200 µ
M TPCK, 200 µ M TLCK, 20 mM NaHSO3, 100 µ g/ml RNAse A, 50 mM Sodium
pyrophosphate, 200 mM NaF, 2 mM ATP, and 200 mM Phosphate pH7.5)
3. Vortex and then centrifuged for 30 min at the top speed of the microfuge.
4. The supernatant was transferred to a tube containing mAb and 20 µ l 1:1 protein A
sepharose slurry, and the tube was rotated end-over-end overnight at 4 oC.
5. The immunoprecipitate was then washed at least 6 times with MES-Salt buffer(20
ml MES pH 6.8, 20 mM NaCl, 1 mM EDTA) for 5 min. each.
6. The beads were pelleted for 2 min. at a microfuge, resuspended into 2 x SDS
sample buffer, boiled for 5 min. at 90 oC sand bath.
8. Run SDS-PAGE.
(P.C., 01/30/95)
Notes:
Instead of 2° GAMIgG can use whole Staph. aureus, Protein A, Protein G which
binds to IgG1 better than Protein A, Prot.A/Prot.G mix (Pierce Immunochemicals), or
antimouse Affigel.
Can release antigen from immunocomplex by 0.1M Glycine pH 2.5 acid shock, or
high salt (3M NaSCN) shock, then passage through Costar Spinex 0.22m m filter
unit into Eppendorf.
Can increase titer of 1° mAb by passing 9E10 media onto Sepharose CNBr beads,
this binds 5 or more Fc portions of the IgG effectively making it an IgM.
Can increase titer of 1° mAb by adding equal volume of saturated NH4SO4 dropwise
to spinning 9E10 media at roomtemp, pelleting the precipitate at 2500g for 5min,
resuspending the pink (RPMI) pellet in dH20, repeating the precipitation.
To make saturated NH4SO4: boil water, add NH4SO4 until crystals fall out of
solution, cool to RT, pH to 7.0 with NH4Cl, filter through 3MM paper.
This protocol takes advantage of the fact that antibodies transfer rapidly between antigen samples
attached to separate solid supports. It allows one to affinity purify small amounts of antibody using less
than a picamole of antigen. This is great for doing immunofluorescence with dirty antibodies that are in
short supply or whose antigens are in short supply, or for quickly screening expression clones for
epitope selection.
For immunofluorescence:
1. Immobilize your antigen on a 1 cm2 chip of nitrocellulose. For example, spot blot
1-10 ng of native Dicty dynein in 10 µ l P100 buffer onto a nitrocellulose chip. This
is your source blot. Make one source blot for every coverslip you wish to stain.
2. Let nitrocellulose dry. Mark the protein side with a pencil. Block in 5% milk/PBS
for 30 minutes. Source blots can be stored in blocking solution in the fridge if NaN3
is added to 0.02%.
1. Grow up dense IPTG-induced (clonal!) phage plates and lift expressed fusion
proteins onto nitrocellulose filters as usual.
2. Block phage filters in 5% milk/PBS for 30 min. Incubate with the antibody for 1-4
hours at the same dilution used to screen the phage library. Wash filters in PBS.
These are your source filters.
3. Run a curtain SDS gel of a sample of purified or enriched antigen. Blot the gel
onto nitrocellulose and mark the protein side with a pencil line across the entire width
of the blot. Block in 5% milk/PBS for 30 minutes and cut into strips.
4. Incubate each source filter to be tested with a strip of curtain gel. Place the source
filter and the blot strip with protein sides facing each other in a seal-a-meal bag. Add
just enough PBS/0.1%BSA to wet both blots. Seal the bag. DO NOT ADD
ANTIBODY AT THIS POINT!
5. Incubate blots together for 1-4 hours. Then remove blot strips and wash
extensively in PBS. Do not mix strips in washing solution or secondary antibody
solution, as antibody may transfer between strips. Incubate the strips in the
appropriate secondary antibody for 1 hour. Wash and develop strips.
6. If a phage clone encodes a truly positive cDNA, the corresponding strip will be
positive as well. Negative strips indicate false positive phage clones.
1/95, Trivinos
Department of Pathology
Center for Immunology
Antigens:
Proteins: 10-100 µg
Cells: 0.5 - 5.0 x107
Adjuvant:
Schedule:
1. Healthy Sp2/0 cells should be rapidly growing by this time. Sp 2/0 cells
should be started about two weeks before the cell fusion. Every two days, they
should be centrifuged at a 64.4 xg on the IEC clinical centrifuge (in 50 ml
tubes) for two minutes. The media should be removed and the cells
resuspended in fresh media. This ensures that only the healthiest cells will fall
to the bottom of the tube. Centrifugation at higher speeds or for longer time
periods should be avoided at this step, because that causes weak or old Sp2/0
cells to precipitate also, and is contra-indicative of what you want to
accomplish.
2. Begin the cell fusion by centrifuging two 50 ml or eight 10 ml flasks of Sp2/0
cells that have been transferred to fresh media one to two days previously, at a
setting of not more than 3 for not more than 3 min in an IEC clinical
centrifuge. Decant the media. You need a ratio of 1:5 healthy, rapidly growing
Sp2/0 to spleen cells. This number of flasks will provide about the correct
number.
3. Remove two spleens from the mice selected above, and place them in washing
media. Tease apart the spleens. Don't be afraid to take two pair of tweezers, or
tweezers and syringe tip and shred the spleens. Then remove cells by
perfusing media through the spleens and also by disrupting portions of the
spleen with the tweezers. Then remove the remaining large chunks of spleens
with tweezers, and place the cells in a 50 ml tube. Centrifuge at a setting of 3
in IEC clinical centrifuge for 3 minutes.
4. Using warm (37oC) washing media, transfer all the cells to one 50 ml tube,
bring the final volume to about 25 to 30 mls, mix by vortexing (THIS IS THE
LAST TIME YOU WILL VORTEX ANYTHING in this procedure ) , and
centrifuge at a setting of 5 for 3 minutes. The objective here is to pack the
cells tightly so that their cell membranes are touching. You also need a large
surface area, and to prevent layering of the large Sp2/0 cells on the bottom and
spleen cells on top. The best tubes to use are the widest, flattest bottomed ones
(our 50 ml conical tubes work fine). The worst tubes are the narrow, very
conical bottomed tubes (our 15 ml culture tubes). If it is necessary to use 15
ml tubes, use round bottom ones only!
5. Add one ml of warm (37o) 50 % PEG (m. wt. 1500) (source and type) over
one minute, gently swirling the tube at 37oC. If you add the PEG with a 1 ml
pipette and gently stir the cells, you will probably obtain many more
hybridomas. After the PEG is added, cap the tube, gently swirl a couple more
times, then centrifuge at a setting of 5 for 3 minutes (minimum). This is the
critical step. Cells must be compacted and stuck together for cell fusion to
occur. This step will also ensure that the PEG comes to the surface while the
cells are compacted at the bottom of the tube. Then remove as much PEG as
possible with a pipette. (CAUTION: PEG is toxic to cells, and should be
removed promptly. This is not the step to "take a break.")
6. Add 8 to 10 mls of warm (37oC) washing media over a period of 2.5 to 3
minutes, again gently swirling the tube. Do not disturb the cell pellet. Add the
media as gentle drops. Remember that the cells are very fragile. After addition
of the media, cap the tube, gently swirl it another time or two, then centrifuge
at a setting of 5 for 3 minutes. Remove the media. This step can be repeated
once more, to ensure that all the PEG is removed, but this appears to be an
optional step.
7. Finally, using a large tipped pipette, such as a 5 ml disposable pipette, and
warm complete media (containing HT media, for the very best results) transfer
the cell pellet to a 50 ml flask. Do not disrupt the cell pellet or use a syringe!.
Hybridomas will grow out of the clumps of stuck-together cells. Allow the
cells to grow in a 50 ml flask in the presence of CO2, HT media, and the
unfused cells, for 4 to 24 hours. It seems that the cells are too fragile to handle
immediately after fusion, but large numbers of hybridomas have been obtained
when cells were plated on the same day as the cell fusion. Cold Spring Harbor
(1989) does not include the overnight incubation prior to plating.
8. Add HAT media to the 50 ml of media in the flask (50x HAT is used at a ratio
of 1 ml/100 ml of media; 500x HAT is used at a ratio of .1 ml/100 ml of
media). Plate the 50 mls into the center 60 wells of 5 96 well plates WITH A
WIDE TIPPED PIPETTE (300 wells) - DO NOT use a syringe and needle!
Cells should cover the bottoms of the wells. This is important to maintain the
CO2 level at a high enough level, and possibly the hybridomas obtain growth
hormones from the unfused spleen cells. The complete media supplemented
with fetal bovine serum should support the growth of 50 cells/well, but ours
does not appear to do this. The first thing one would consider, is that the fetal
bovine serum content is too low, but our media supports the growth of Sp2/0
and established hybridoma cells very well. The problem here appears to be the
CO2 content. Therefore, high cell density maintains the CO2 at a higher level,
and more hybridomas survive.
9. After 4 to 5 days, add complete media supplemented with HT to the wells.
10. After 1 week, test the wells with hybridomas against the antigen by an ELISA.
11. Expand positive hybridomas into 24 well plates. You MUST use spleen feeder
cells and HT media. If many wells are positive, hybridomas may be combined
into expansion wells. CELLS MUST BE RE-EXPANDED EVERY TWO
TO THREE DAYS. Biochemistry book recommends that hybridomas be
cloned immediately, in order to prevent overgrowth of the desired cells, by
non-secreting cells that may be present.
Summary:
The mouse is immunized six times. After the spleen is removed, the splenocytes are
obtained and fused with myeloma cells using PEG. The hybrids are plated into 96
well tissue culture plates and observed for colony growth.
OUTLINE
PROTOCOL