Arthritis, Degenerative Clinical Trial
Official title:
Use of Autologous Adipose-Derived Stromal Vascular Fraction to Treat Osteoarthritis of the Knee
Autologous adipose-derived stromal vascular fraction (SVF) was used to treat 10 osteoarthritic knees of grade II or III (K-L scale) under IRB-approved protocol in a feasibility and safety study. The adipose-derived SVF was obtained through disaggregation of lipoaspirate and resuspension of the SVF in 3 ml of Lactated Ringer's Solution, with a mean of 48 million nucleated SVF cells and a mean viability of 78%, injected per knee. Cell suspension was injected into the intra-articular space using ultrasound guidance. At 12 weeks post-op all 10 knees showed decreased pain and increased mobility, both statistically significant (α = .01). Nine of ten knees reported either maximum possible or very significant decrease in pain. No infections, acute pain flares, or other adverse events were reported. Patient ages ranged from 52 - 69 years with a mean of 59 years.
Methods:
Adipose Harvest. Using no oral or parenteral sedation, standard wetting solution (1 liter
Lactated Ringer's, 50 milligrams of 1% lidocaine, and 1 cc of 1:1000 epinephrine) was
infused through small incisions created with the tip of a #11 scalpel blade in the abdomen
or flank using a standard multi-hole infusion cannula. A super-wet plus technique (2 volumes
of wetting solution to 1 volume of proposed fat aspirate) was used to infuse the solution
into the deep and superficial fat compartments. Twenty minutes was allowed for maximum
vasoconstrictive effect of the epinephrine. Fat was harvested using standard
Suctioned-Assisted Liposuction (SAL) method with a 3mm cannula at approximately .5 - .7
atmosphere of vacuum, aspirating approximately 200-300 cc of lipoaspirate into a sterile
tissue processing container (GID SVF-1, Lousiville, CO) for each knee to be treated.
Adipose processing method. Lipoaspirate was harvested and processed all the way to the
generation of the SVF within a single GID SVF-1 sterile disposable device. The GID SVF-1
unit contains the washing mechanism, the mesh filter, and the centrifuge capability in the
same device. After harvest the lipoaspirate was washed three times with 37C Lactated
Ringer's Solution with 20 mg Cipro and 5,000 units heparin per liter and the fluid portion
removed using the mesh filter system, leaving dry adipose inside the canister. The canister
was weighed to determine the amount of dry adipose available for further processing. The
washed adipose was disaggregated using Type I collagenase (Worthington, Lakewood, NJ) at a
concentration of 200 CDU/ml of total catalytic volume where total catalytic volume is the
volume of the adipose tissue plus an equal volume of 37C Lactated Ringer's Solution. The
collagenase was injected into the canister through a sterile .22 micron filter (Millex-MP,
Millipore, Cork, Ireland). The device with adipose, buffer, and collagenase was then placed
into an incubated shaker for 40 minutes at 38C at 150 RPM, see Figure 1. After
disaggregation human albumin solution was added to achieve a concentration of 2.5% and stop
any further collagenase activity. The device was then centrifuged at 800 g for 10 minutes.
The supernatant, including all floating cells and debris and the aqueous phase, was removed
using a port on the top of the device and discarded. The SVF pellet at the bottom was
resuspended in 10 ml of sterile LR accessed via the central port on the device using a 14G
5.5 inch spinal needle (Abbocath-T, Hospira, Sligo, Ireland). A sample of 0.5 ml of the
resuspension was collected in a 1.5 cc Eppendorf tube to be used for cell counting and
assay. The resuspended SVF cells were concentrated into a 3 ml dose using a sterile 15 ml
Falcon tube at 400 g for 4 minutes.
SVF counting method. The SVF cell count and viability was assessed using an ADAM MC image
cytometry system (Bulldog Bio, Portsmouth, NH). The ADAM MC uses propidium iodide staining
to count viable and non-viable nucleated cells. A 100 µL aliquot of the assay sample was
diluted with a 1:5 ratio (1 part sample to 5 parts sterile LR) to adjust the sample within
the operating limits of the ADAM MC. The differential stains were applied and aliquots
loaded into the disposable cassette that is utilized with the ADAM device. The results from
the ADAM counting device provide the concentration of SVF cells in the resuspension syringe
and the percentage viability. The total volume of the resuspension in the syringe was
multiplied by the concentration to give the total number of resuspended mononucleated cells
(no adipose cells, no RBCs, and no fragments included in the counting process).
Injection and image guidance method. The patient was placed in the supine position and the
area over the lateral suprapatellar region of the knee was prepared in the usual sterile
fashion using an iodine prep solution (1% Iodophor) followed by a 70% Isopropyl Alcohol
solution. This location was used due to ease of access into the intra-articular space and to
avoid injecting into the fat pad of the knee. No sedation or pain medication was
administered to the patient. An ethylchloride topical anesthetic was sprayed on the lateral
knee until the skin color changed to white. Lidocaine local anesthetic was injected using a
25 gauge needle to numb the skin and subcutaneous tissues. Using an M-Turbo Sonosite
ultrasound system, the joint space was identified and under live ultrasound guidance the
knee was aspirated using an 18 gauge/1.5 inch needle, if fluids were available for
aspiration. Then all of the 3 cc of buffered solution of SVF was slowly injected into the
intra-articular space through the same 18 gauge/1.5 inch needle. The needle was then be
removed and direct pressure over the injection site will placed for approximately ten (10)
seconds. Hemostasis after injection was confirmed, and then the injection site was cleaned
with an alcohol wipe and covered with a sterile band-aid. The patient was given crutches and
asked to be non-weight bearing on the injected knee for two (2) days. The patient was
allowed to bend and flex the knee as long as non-weight bearing condition is maintained.
Pain and mobility assessment methods. Assessment of knee pain was done using the PROMIS pain
instruments, a validated pain scale system developed under funding by the NIH. PROMIS
(Patient Reported Outcomes Measurement Information System) is a system for measures of
patient reported health status for physical, mental, and social well-being, including three
measurements of pain (www.nihpromis.org). The PROMIS Pain Intensity instrument (3a) assesses
how much a person hurts. The PROMIS Pain Behavior instrument (Bank 1.0) measures behaviors
that indicate to others that an individual is experiencing pain. The PROMIS Pain
Interference instrument (Bank 1.0) measures the consequences of pain on relevant aspects of
one's life. Patient responses are converted to numeric values in a validated scale.
Responses to each question in a pain instrument range from 1 to 5 (1=not at all, 2=a little
bit, 3=somewhat, 4=quite a bit, 5=very much), and are summed over the number of questions in
the bank to create a raw score. The raw score is converted to a standardized score using an
iterative response method with a mean of 50 and SD of 10, based on a large sample of the
general population of the United States. The validated PROMIS pain scales provide interval
data and allows calculation of the mean and SD, and use of t-tests of significance. Data was
recorded pre-operatively (time 0), and at follow-up points at 2 weeks, 4 weeks, 6 weeks, and
12 weeks.
Additionally patients were asked to respond to a pain and mobility questionnaire with one
question on pain and one question on mobility. The questionnaire asked the patient to
compare their increase/decrease in pain and mobility relative to before surgery, using a ±
1-5 scale, see Figure 2. On this scale negative numbers correspond to decreasing
pain/mobility, and positive numbers correspond to increasing pain/mobility. This
questionnaire provides ordinal data and allows calculation of the median and significance
using Wilcoxon Ranked Sums nonparametric testing.
;
Endpoint Classification: Safety Study, Intervention Model: Single Group Assignment, Masking: Open Label, Primary Purpose: Treatment
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