Breeding
Soundness Examination of the Dog
 287-298
Identification
- The identification is not only important for
the medical records, but is essential in the case of a pre-purchase
examination.
- Failure to positively identify an animal could
cause legal problems in the future.
History
- Has the dog ever been bred?
- Has he ever sired a litter? If has bred, but
never sired a litter, you may consider congenital infertility.
- If he has sired litters, and is now infertile
you may consider acquired infertility.
- Frequency of use
- Every other day breeding is usually
acceptable.
- Breeding more than that may be overusing the
dog.
- Has there been any exogenous drug therapy
(testosterone etc.)?
- What is the dog's habitat?
- Is he in a kennel?
- Is he housed with bitch? If so, the bitch may
be dominant.
- Is he 'mommies little boy', who has not had any
canine contact?
- Has he had any exposure to sex?
- Has he been punished for showing sexual
interest?
- Has his libido changed?
- Has he ever been shown?
- Does he have any endocrine disease?
Physical Exam General
exam
- Look for signs of endocrine problems.
- Check for any congenital disorders that would
make him an unsuitable potential breeder.
- Reproductive Exam
Testes
- Check for shape, size, and consistency.
A
bad way to measure dog testes.
A
good way to measure dog testes.
- Testicular asymmetry can be indicative of
testicular degeneration.
- The normal size of the testes can be estimated
using the equation:
- log Scrotal Width = 0.324(log Body Weight) +
1.249
- Check to make sure he is not cryptorchid.
- The
testes should be present by 16 weeks.
- You can give them 6 months,
but they probably will not descend.
- There is generally no acceptable
treatment, but hCG is cited to help (100-1000 IU 2 times/week for 2
weeks) at less than 16 weeks of age
- Check
this link out about testicular prostheses for those of you who are
unscrupulous!
Penis
- Check for abnormalities, including:
- Blood
- Trauma
- Tumors
- Paraphimosis
- Short Sheath
- Phimosis
- Short Penis
- Stricture
- Priapism - Seen
with Spinal Injury
- Os Penis -Fractures,
Congenital Abnormalities
- B. canis - covered in bitch notes.
The Brucella
canis status of the male should be
ascertained. The rapid slide agglutination test has many false
positives and a true positive titer may wane over time.
Semen collection
- It is recommended that the dog have five days
of sexual rest before obtaining a semen sample for evaluation.
-
Conversely, if the dog has not ejaculated within ten days, a higher
than normal number of detached heads and distal droplets will be
seen because of prolonged storage.
- This problem will normally
resolve if a second ejaculate is collected.
Method
Hand collection
or
manual
stimulation
Click to see 'semen collection'
- Use a rubber cone and collection tube or a
disposable plastic cone with end sealed.
 
- Slide the prepuce over the bulbous glandis.
(Erection normally occurs after intromission into the vagina.)
- Slide
the cone over penis and apply a gentle 'stoke' pressure to penis, bulbous.
- Three portions to ejaculate
- Pre-sperm is the clear, first portion seen
during the initial thrusts.
- Sperm rich -
White portion seen during thrusts.
- Prostatic portion
- Clear portion seen when thrusting is
done. It may be seen after the 'stepover', when the dogs are rear to
rear.
- The prostatic portion is not needed for
fertility. It
can be collected to evaluate the prostate.
Problems with collection
No interest by male
- An estrus bitch is helpful for collection.
- Sperm numbers have been found to be greater if
an estrual bitch is present.
- You can give estrogen to ovariectomized bitch,
but there are potential problems doing this.
- You can use the dog pheromone, hydroxy benzoic
acid, or ICG's 'Eau d' Estrus', or frozen swabs from an estrual
bitch.
 Recent work
from VPI shows that 0.1 mg/kg PGF2alpha 15 minutes prior
to semen collection significantly increased sperm output over that
of saline or GnRH or oxytocin treated males. No comparisons were
made with estrual bitches.
- The swabs usually give a better response than
synthetic chemicals. These attempts may help, or may not.
- There may be technique problems in the
collectors performance, such as being too vigorous or not vigorous
enough.
- The dog may be in an unfamiliar environment,
such as a clinic. The distractions at a clinic include the smells,
noise, and 'gapers'.
- It may be better to not have the owner present,
or it may be better to have the owner present, or it may make
difference at all.
- Poor sexual experience, pain with sex resulting
from orchitis, prostatitis, lumbar and stifle pain may hinder
collection.
Semen
evaluation
- At the 1992 Annual Meeting of the Society for
Theriogenology, guidelines for the breeding soundness examination of
the dog and a canine semen evaluation form were introduced.
- The first step in semen evaluation is to
examine the color of the different fractions (Fraction 1 - F1,
Fraction 2 - F2 and Fraction 3 - F3). F1 and F3 should be clear,
whereas F2 should be cloudy.
- Yellow, brown or red samples may indicate the
presence of urine or blood, respectively.
- Always remember to use warm slides and
equipment when examining semen samples for motility.
- A cytologic examination of the non-sperm cells
(F2 and F3) can be made by smearing a drop of semen and staining it
with modified Wright's (e.g. DiffQuick). White cells indicate an
inflammatory process and a culture may be indicated.
- RBC
- WBC
- Macrophage -
associated with azoospermia
| |
Whole Ejaculate |
F1 |
F2 |
F3 |
| Color |
Opaque/White |
Clear |
White |
Clear |
| Volume (mL) |
< 35 |
0.25-3.0 |
0.4 - 3.0 |
1.0 - 2.0 |
| pH |
6.1 - 7.0 |
8.2 - 8.4 |
6.1 - 8.9 |
6.5 - 8.7 |
| Conc (106/mL) |
65 (10-200) |
|
|
|
| Total Sperm (106) |
390 (200 acceptable) |
|
|
|
| Total Motility |
> 70% |
|
|
|
| Progressive Motility |
> 80% |
|
|
|
| Velocity |
Fast |
|
|
|
| Normal cells (%) |
>80% |
|
|
|
- The standards set forth by the Society for
Theriogenology are not absolute and do not guarantee fertility or
sterility, but are set forth as guidelines for the practicing
veterinarian to use as a standard method to evaluate a dog's
potential fertility.
- Canine semen evaluation forms are available
from the Society for Theriogenology.
Breeding with Fresh Semen
-
Artificial Insemination
requires no special treatment of the semen
-
Always examine the ejaculate
-
The prostatic portion
is not needed - you may want it to increase the volume
-
You may want to extend
to have an easier volume to handle (usually do not want more that
5 to 6 cc.
-
Volumes
as low as 2.2 ml and up to 3.6-3.9 ml have been reported to
yield good pregnancy rates.
-
Conception rates
should be around 90% if the bitch is bred every other day while in
estrus
-
At
least 220 x 106cells
need to be inseminated to achieve optimum fertility.
-
Vaginal
AI on 3 consecutive days after acceptance of the male by the
female using 50 x 106 spermatozoa in fresh semen
extended 1:4 for each breeding resulted in lower fertility
(20%) than AI on 3 consecutive days with 200 x 106 cells
of fresh semen extended 1:1 (80%) or natural mating (80 %).
-
Vaginal AI is
suffcient
-
It
has been shown that if AI is performed twice, rather than once,
around the time of best fertility conception rate is significantly
improved.
-
There
also appeared to be a trend toward increasing pregnancy rates when
the number of inseminations increased
-
Transcervical breeding
when the dogs have normal fertility is not needed
-
Transcervical breeding
has been shown to help when fertility is low
Breeding with Chilled Semen
-
AKC requires the proper paperwork
to be completed, as well as DNA identification of the stud and the
bitch before a litter can be registered.
-
Ovulation timing in the bitch is
critical
-
It may take 1-2 weeks to train a
male to ejaculate in a veterinary office without an estrual bitch
present. Therefore, it is ideal for the dog to have had semen
collected and to be familiar with the collection procedure long before
any semen is actually needed.
-
It is also advisable to prepare a
“test shipment” in advance.
-
A semen sample should be
extended, stored a minimum of 24 hours in the container that will
be used for transport, and evaluated after 24 hours to ensure that
extension and storage do not have detrimental effects on the semen
quality.
-
Not all males’ semen
will respond to extending, cooling and storage in a similar
fashion, and this ‘test shipment’ will determine the viability
of the sperm after extension and cooling.
-
Not only must the male be trained,
but also shipping company schedules and venues to which they ship need
to be carefully assessed well before the need arises.
-
Some destinations are
serviced by shipping companies and some are best served by
counter-to-counter airline shipments.
-
In some cases shipments
cannot be sent out on the appropriate day and in others
shipments cannot be delivered on the appropriate day.
-
Semen is analyzed
-
Extension
-
Appropriate
semen extender is added to the ejaculate, usually 1:1.
-
Semen
extenders provide an energy source and buffers that enhance the
survival of chilled sperm cells.
-
Extenders
can be obtained from commercial sources that are manufactured
exclusively for extending canine semen (Synbiotics, San Diego, CA
92127; CLONE, Chester Springs, PA 19425; Camelot Farms, College
Station, TX 77842; International Canine Semen Bank, P.O. Box
651,Sandy, OR 97055),
-
Equine
semen (Lane Mfg., Denver, CO 80231; IMV Intl, Minneapolis, MN
55430) work well and are much cheaper.
-
Homemade
semen extenders can also be prepared, however proper laboratory
techniques
-
The
extender must be pre-warmed before adding it to the semen or the
spermatozoa will suffer cold-shock.
-
The
prostatic portion of the ejaculate may have detrimental effects on
the storage of canine sperm cells,
-
We
found no detrimental effects on pregnancy rate or fecundity when
whole ejaculates were extended 1:1 and inseminated after 24 or 48
hours of storage.
-
If
the entire prostatic portion of the ejaculate is collected and the
semen is extended, the volume of the resulting extended semen may
be such that it cannot be completely inseminated without some
vaginal reflux.
-
LSU research (EVSSAR 2007 Estoril, Portugal)
-
Semen collected from 6 dogs and extended in INRA 96 for horses
-
Diluted 1:1 and:
-
Prostatic fluid and centrifugation have no effect on the membrane integrity of the cells when semen is extended in a commercial equine extender.
-
Semen extended should have the prostatic fluid removed before storage and it should be stored at a relatively high concentration.
-
If a sample does arrive that has a large volume because the prostatic portion was included in the extended semen, centrifugation to remove the prostatic fluid yields progressive motility that is not different from removing the prostatic fluid before extension.
-
Containers
-
Containers
designed to ship semen can be obtained from many of the same
sources that provide canine semen extenders. (Synbiotics, San
Diego, CA 92127; CLONE, Chester Springs, PA 19425; Camelot Farms,
College Station, TX 77842; Bio-Flite, Anaheim Hills, CA 92807;
International Canine Semen Bank, P.O. Box 651, Sandy, OR
97055).
-
The
containers usually consist of a Styrofoam box, an ice pack, and
container for the semen.
-
These
commercially available semen containers maintain semen well enough
that acceptable pregnancy rates result.
-
Commercially
available shipping containers offer a predictable, attractive and
easy way to ship semen.
-
Many
of these containers are relatively expensive when compared to the
disposable equine shipping containers.
-
A
commercially available (although no longer marketed)
disposable equine shipping container allowed storage of
extended canine semen for up to 48 hours and the resulting
pregnancy rates were equivalent to AI with fresh semen.
-
We
have used other brands of
disposable equine semen
shippers and have had good success in maintaining semen
viability.
-
The
advantage of the equine shippers is their lower cost than the
canine semen shippers
-
The
semen need not be warmed prior to AI.
-
It
is recommended to save a small aliquot of the semen for evaluation.
-
Results
-
Same as natural breeding if
sufficient spermatozoa are inseminated at the proper time.
-
Vaginal AI on 3 consecutive
days with 200 x 106
cells/breeding
with semen extended 1:1 and stored for 24 hours gave the same
pregnancy rates as natural mating using the same breeding schedule
(80%),
-
Using
50 x 106 cells extended 1:4 and stored for 24
hours resulted in lower fertility (20%).
-
Reports from Sweden that
summarized data from chilled semen inseminations show pregnancy
rates can vary from 28-60% depending upon the type of extender
used.
-
Pregnancy rates are lower when
ovulation is timed and the number of breedings is limited compared
to the 90-100% conception rates when an average of 3.9 breedings
of 250-350 x 106 cells/breeding
were used by us.
Frozen Semen
-
AKC requires the proper paperwork
to be completed, as well as DNA identification of the stud and the
bitch before a litter can be registered.
-
Semen FreezingA
simple method to freeze canine semen that is currently used by the
authors’ laboratory is as follows:
-
After
the semen is collected, a complete analysis is performed.
-
During
the evaluation process, the semen is diluted 1:1 using a
commercially available semen refrigeration extender (Refrigeration
Media - TEST Yolk Buffer (TYB) - 9972 - Irvine Scientific, Santa
Ana, CA 92705-5588) and centrifuged for 10 minutes at 900 x
gravity.
-
After
centrifugation the supernatant is removed and the pellet is
resuspended to a concentration of 400 x 106 cells/ml
using the same refrigeration extender.
-
This
standardized semen sample is then placed in a 5o C
refrigerator for one hour.
-
During
the hour of cooling, an appropriate number of 0.5 ml French straws
are labeled with all the data required by the dog’s registry
(name, registration number, breed, date, collection facility,
etc.).
-
After
one hour, a commercial freezing extender containing 12% glycerol
(Freezing Medium - TEST Yolk Buffer (TYB) with Glycerol - 9971 -
Irvine Scientific, 92705-5588) that has also been kept at 5o
C is added to the cooled semen solution
at 1:1, v:v, to make a final concentration of
200 x 106 cells/ml containing 6% glycerol.
-
In
a 5o C cold box, the 0.5 ml straws are then filled and
the ends are sealed.
-
The
straws are then placed on a screen that is attached to a 3 cm
thick Styrofoam frame, which is floating in liquid nitrogen.
-
After
10 minutes, the straws are plunged into the liquid nitrogen before
storage.
-
Frozen
semen storage
-
Semen is stored at -196o C in commercially available liquid nitrogen tanks.
-
Storage and inventory are critical aspects of frozen semen use. Meticulous records must be kept as to the location and number of straws frozen from each male.
-
The liquid nitrogen must be routinely monitored to ensure that there is sufficient liquid nitrogen to maintain the temperature at -196o C. If frost starts to accumulate on the tank, the semen should be transferred immediately to a new tank and the damaged tank discarded.
-
Most dog breed associations are not as concerned about the quality of the frozen semen as they are about identification of the semen. The quality control of the final product is dependent upon on the integrity of the freezing facility.
-
Frozen semen is usually shipped in ‘dry dewars’.
-
These are small tanks that do not contain any liquid nitrogen, but keep the sample at -196o C for a short (e.g. 1 to 2 weeks) period of time.
-
Since there is no liquid in the tanks, the airlines and shipping companies will allow their shipment, unlike liquid nitrogen tanks.
-
If a liquid nitrogen tank is available at the shipping destination, the semen may be shipped well in advance and transferred to the liquid nitrogen tank upon arrival.
-
If, however, a liquid nitrogen tank is not available at the insemination site, shipment should be timed in accordance with the intended date of insemination.
-
Thawing
-
Thawing
procedures for frozen semen vary as much as freezing
protocols.
-
We
thaw straws at 50o C for 10 seconds.
-
Some
facilities recommend thawing at lower temperatures for a longer
time
-
Some
recommend adding thawing media during the thaw.
-
Best
to use the freezing facility’s recommendation
-
Insemination
technique
-
Vaginal
-
Laparotomy
-
Lapasoscopy
-
Norwegian
-
Fertility
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