Surgical Procedures and Methodology for a Preclinical Murine Model of De Novo Mammary Cancer Metastasis

Podsumowanie

Pre-clinical models evaluating adjuvant therapy targeting breast cancer metastasis are lacking. To address this, we developed a murine model of de novo pulmonary mammary adenocarcinoma metastasis, wherein therapies administered in the adjuvant setting (post surgical resection of primary tumors) can be evaluated for efficacy in impacting previously seeded pulmonary metastases.

Streszczenie

A rate-limiting aspect of transgenic mouse models of mammary adenocarcinoma is that primary tumor burden in mammary tissue typically defines study end-points. Thus, studies focused on elucidating mechanisms of late-stage de novo metastasis are compromised, as are studies examining efficacy of anti-cancer therapies targeting mediators of metastasis in the adjuvant setting. Numerous murine mammary cancer models have been developed via targeted expression of dominant oncoproteins to mammary epithelial cells yielding models variably mimicking histopathologic and transcriptome-defined breast cancer subtypes common in women¹. While much has been learned regarding the biology of mammary carcinogenesis with these models, their utility in identifying molecules regulating growth of late-stage metastasis are compromised as mice are typically euthanized at earlier time points due to significant primary tumor burden. Moreover, since a significant percentage of women diagnosed with breast cancer receive adjuvant therapy after surgical resection of primary tumors and prior to presence of detectable metastatic disease, preclinical models of de novo metastasis are urgently needed as platforms to evaluate new therapies aimed at targeting metastatic foci. To address these deficiencies, we developed a murine model of de novo mammary cancer metastasis, wherein primary mammary tumors are surgically resected, and metastatic foci subsequently develop over a 115 day post-surgical period. This long latency provides a tractable model to identify functionally significant regulators of metastatic progression in mice lacking primary tumor, as well as a model to evaluate preclinical therapeutic efficacy of agents aimed at blocking functionally significant molecules aiding metastatic tumor survival and growth.

Wprowadzenie

Women in North America have a ~12% lifetime risk of developing breast cancer²; a majority of these individuals will have primary tumors removed via surgery, and depending on cancer subtype, will then receive targeted, endocrine, chemo- and/or radiation therapy in the adjuvant setting³. Examples include, women diagnosed with hormone receptor-positive cancers receiving anti-estrogen therapies and women with HER2-positive tumors receiving HER2-targeted therapies with radiation/chemotherapy, whereas no targeted therapies are yet available for triple negative tumors³. Despite advances in radiation, chemotherapy, personalized and hormone-based therapies that supplement surgical resection, disease recurs in 30-70% of women diagnosed with stage II or III disease⁴, as therapies are largely ineffective in eradicating metastatic disease in distant organs, including lung, bone, brain and/or liver⁵. This is especially significant given that when metastatic disease occurs in the absence of primary tumor regrowth, this implies that disseminated malignant cells were likely already present in secondary organs at the time of definitive surgery. Thus therapies able to eradicate or slow growth of metastatic tumors are urgently needed.

While de novo mouse models of mammary carcinogenesis have been remarkably informative in revealing mechanisms regulating neoplastic progression¹, existing models also have several limitations. One of these is the fact that de novo transgenic models typically develop primary tumors in multiple mammary glands, wherein primary tumor burden limits duration of studies. While primary tumor cell escape and metastatic seeding likely occur early in neoplastic progression in these models, frank development of metastatic tumors occurs late, and depending on the mouse model and strain background, is often partially penetrant¹. This further limits the utility of de novo models for discovery of molecules regulating metastasis in secondary organs, and for evaluating preclinical efficacy of therapeutics in the adjuvant setting.

To circumvent these limitations, we developed a de novo autochthonous model of mammary carcinoma metastasis to lungs. Parental transgenic females (i.e., MMTV-PyMT on the FVB/n strain background for studies described herein) bearing late-stage de novo mammary tumors are aged to ~100 days⁶, at which point their primary tumors are surgically resected and enzymatically dissociated into single cell suspensions. Suspensions (1 x 10⁶ cells) are in turn orthotopically explanted into 6-7-week-old recipient syngeneic female mice, where single primary mammary tumors develop over a 38 to 60 day period (Figure 1A). At a defined tumor size (172 to 450 mm³), recipient mice are anesthetized and primary tumors are surgically resected such that tumor regrowth at the surgical site is minimized, consistent with surgery in women (Supplementary Figure 1). On the FVB/n strain background, mice develop histologically-detectable metastatic foci in lungs with 45% penetrance by ~115 days post-surgery (Figure 1B). With this extended latency of metastatic tumor growth, the model is uniquely positioned for adjuvant therapy delivery, and for elucidating and evaluating underlying biology influencing metastatic progression following surgical removal of primary tumors.

Protokół

Animals used in the following protocol are covered by Oregon Health & Science University's Institutional Animal Care and Use Committee (IACUC), which is designed to be compliant with the Animal Welfare Act regulations and Public Health Service (PHS) Policy.

Maintenance of sterile conditions: Sterilized instruments should be used and between mice, should be wiped clean with sterile gauze, rinsed in PBS followed by sterilization with disinfectant 70% ethanol for at least 15 minutes. A surgical cap, facemask, gown, and gloves should be worn for survival surgeries. Pre-operative preparation of the animal for survival surgeries is included in the following protocol. Refer to Table 1 for a list of reagents and equipment.

1. Isolation and Preparation of Single Cell Suspensions from Primary Mammary Tumors

1. Anesthetize donor female 100 day old transgenic MMTV-PyMT (FVB/n) mice and maintain under continuous sedation by administering 2% isoflurane via an anesthesia mask. Confirm that the mouse is properly anesthetized with an absent foot pinch reflex.
2. In a sterile setting, resect primary mammary tumors from 100-day old transgenic female MMTV-PyMT (FVB/n) mice by separating mammary tumor from overlying skin and surrounding adipose tissue and/or lymph nodes using sterile scissors. Euthanize the anesthetized mice by cervical dislocation.
3. With sterile scissors or a scalpel, mince primary tumors manually into small pieces (~1.0 mm³). Place tumor pieces in 3.0 mg/mL collagenase A and 4.0 U/mL DNase I dissolved in DMEM. Use ~10 mL of the above digestion medium per 1.0 cm diameter tumor.
   1. Perform digestion in a sterile 25 mL bottle with a sterile stir bar at ~125 rpm and 37 °C for 40 min.
4. Stop the digestion by adding fetal bovine serum (FBS) to a final dilution of 10% and place the entire mixture on wet ice where it is maintained.
5. Filter the digested tumor suspension through a 0.7 µm nylon strainer into a 50 mL conical tube and discard any tumor remaining in the strainer. Centrifuge the supernatant at 300 x g at 4 °C.
6. Resuspend the pellet in 10 mL DMEM per 1.0 cm tumor and re-filter through a 0.7 µm nylon strainer. Count cell concentration, then centrifuge at 300 x g at 4 °C.
7. Resuspend pellet in 10% dimethyl sulfoxide with 90% FBS at a concentration of 2 x 10⁷ live cells/mL. Store single-cell suspensions of whole primary tumor at -80 °C.

2. Orthotopic Injection of Mammary Tumor

1. Partially thaw frozen primary tumor suspensions at 37 °C until the frozen pellet can be released from the cryogenic tube into 20 mL DMEM and count the cells. Centrifuge at 300 x g at 4 °C and resuspend cells in a 1:1 DMEM: growth factor-reduced solubilized basement membrane preparation extracted from the Engelbreth-Holm-Swarm (EHS) mouse sarcoma at a concentration of 1 x 10⁷ cells/mL (see the Table of Materials).
2. Place the anesthetized recipient female syngeneic mouse ventral side up and maintain under continuous sedation by administering 2% isoflurane via an anesthesia mask.
3. Sterilize the right 4th mammary gland injection site using aerosolized 70% ethanol and applying Poly(vinylpyrrolidone)-Iodine with a sterile cotton swab.
4. Inject 100 µL (1 x 10⁶ live cells from frozen primary tumor suspensions) bevel-side up into uncleared right 4th mammary gland of the 6 to 10 week-old female FVB/n mouse using a 29 G 0.3 mL insulin syringe.

3. Surgical Resection of Orthotopic Mammary Tumor

1. 38-60 days following tumor cell injection, euthanize mice not exhibiting orthotopic tumor volumes ranging between 172 to 450 mm³ in volume [length x (width²)/2] (about 75% of injected mice).
2. Place anesthetized mice displaying proper tumor size ventral side up under continuous sedation by administering 2% isoflurane via an anesthesia mask and confirm the mouse is properly anesthetized with an absent foot pinch reflex. Apply vet ointment to the eyes for prevention of dryness while under sedation.
3. Spray 70% ethanol to sterilize the surgical area surrounding the primary tumor, then apply Poly(vinylpyrrolidone)-Iodine with a sterile cotton swab.
   NOTE: Hair removal at the surgical site resulted in skin excoriations and/or infections for ~5% mice and was therefore excluded from this step (data not shown).
4. As shown in Figure 1C, make an initial skin incision using blunt scissors medial-caudal to the tumor.
5. Next, make a superior excision of the skin (Figure 1C) medial to the tumor. Pay attention to the need to cauterize any vasculature feeding the tumor located on the skin before extending the incision.
6. Continue the skin incision laterally (posterior to the tumor), then make a superior skin excision (lateral to tumor), and medial excision (superior to tumor) (Figure 1C).
7. After the skin has been excised circumferentially around the tumor (Figure 1C), lift overlying skin attached to the tumor using forceps while blunt dissecting the tumor away from the abdominal wall musculature and keeping the mammary glands intact.
8. Identify (by blunt dissection) and cauterize large vessels running through the 4^th and 5^th mammary glands.
9. Excise approximately half of the 4^th and 5^th mammary glands at the cauterization site to free the tumor, overlying skin, and segments of the mammary glands (Figure 1C).
10. In the event of bleeding, identify actively bleeding vessels and immediately cauterize them. If more than 250 µL of blood is lost, exclude the mouse from study and euthanize it.
11. Close excision sites with wound clips using a wound clip applier (Figure 1C).
    NOTE: Remove the wound clips 10 days post-surgery with a wound clip remover.
12. Administer warm sterile saline subcutaneously (4% of the animal's body weight) and keep the animal warm with a heat lamp. Check the animals every 5-10 min during recovery from anesthesia.
    NOTE: Administration of either bupivacaine or lidocaine increased post-operative mortality (data not shown). Mice that showed signs of pain (hunching, unwilling to move, failure to groom) 1 h after surgery were euthanized.
    1. Once the mouse has fully recovered, return it to the company of other mice.

4. Isolation and Processing of Blood and Lung for Flow Cytometry and Histology

1. At the study endpoints, prepare mice for various histopathologic assessments if desired. 90 min before euthanasia, give each mouse an intraperitoneal injection of bromodeoxyuridine (BrdU, 50 µg/g mouse weight) at a concentration of 6.25 µg/µL in 1x PBS.
   NOTE: Frozen stocks of dissolved bromodeoxyuridine are used within 1 month after preparation.
2. 10 min before euthanasia, with the mouse anesthetized, collect retroorbital blood (>500 µL) using heparinized capillary tubes, and subsequently transfer to tubes coated with dipotassium EDTA held on ice.
3. To remove lungs and remaining mammary tissue, make a midline incision with scissors from the lower abdomen to the mouth to expose the thoracic and peritoneal cavities (Figure 2A), and peel the skin laterally to also expose the remaining right 4^th and 5^th mammary glands.
4. Excise the remaining mammary gland tissue and examine it to rule out primary tumor regrowth by assessing serial sectioned formalin-fixed paraffin-embedded (FFPE) tissue by hematoxylin and eosin (H&E) staining (Supplementary Figure 1).
5. To remove lungs, open the abdominal wall to the diaphragm with scissors, then euthanize the animal by cutting the abdominal aorta to drain blood prior to perfusion of lungs (Figure 2B-2C).
6. Cut the diaphragm along the rib cage from an abdominal approach making sure to avoid the lung and heart. Then, expose the thorax by cutting through the lateral sides of the rib cage (Figure 2D).
7. Using a 23-gauge needle on a 20 mL syringe, perfuse lungs with ~5.0 mL DPBS (~10 mL/min) through the right ventricle of the heart until the lungs turn entirely white (Figure 2E-2F). Immediately cut off the heart from the main vessels so blood does not re-perfuse into the lung.
8. For lung tissue to be fixed and processed for histopathologic assessments, inject ~1.0 mL 10% formalin at 4 °C into the exposed trachea bevel side up toward the lungs using a 23-gauge needle (Figure 2G-2H). Cease injection once lungs are completely expanded and filled with fixative (Figure 2I).
9. Excise lung lobes from trachea, and emersion fix lung tissue in neutral-buffered formalin for subsequent paraffin embedding or OCT-freezing medium, per standard histopathologic procedures.
10. Quantitatively evaluate metastatic burden in lungs by serial sectioning of FFPE lung tissue and evaluate microtome sections (100 µm, thirteen sections), by H&E staining (Figure 1B).

Wyniki

Greater than 75% of recipient mice receiving 1 x 10⁶ cells from primary mammary tumors derived from MMTV-PyMT mice, develop single mammary adenocarcinomas ranging in size from 172 to 450 mm³ within 38-60 days (data not shown). Mice eligible for randomization are then enrolled into study groups following surgical resection of primary tumors as shown (Figure 1C). Primary tumor regrowth was identified in less than 2% of mice that underwent ...

Dyskusje

Modifications and troubleshooting:

When blunt dissecting tumor away from the abdominal wall, the tumor may remain adherent to the abdominal wall. This was observed in <5% of mice injected with tumor (data not shown). For mice with tumors adherent to the abdominal wall, the mouse should be euthanized as resection is difficult without primary tumor regrowth.

Limitations of model/technique:

Whereas other...

Materiały

Name	Company	Catalog Number	Comments
Isofluorane	Piramal Healthcare	N/A	Prescription order
Collagenase A	Roche	11088793001
DNase I	Roche	10104159001
DMEM	ThermoFisher	12634010
25 mL Pyrex bottle	Sigma-Aldrich	CLS139525
Fetal Bovine Serum	Atlanta Bio	S11150
0.7 µm nylon strainer	Corning	352350
50 mL conical tube	VWR	89039-658
Dimethyl sulfoxide	Sigma-Aldrich	D2650
Growth factor-reduced Matrigel	BD	354230	Growth factor-reduced solubilized basement membrane preparation extracted from the Engelbreth-Holm-Swarm (EHS) mouse sarcoma
Poly(vinylpyrrolidone)–Iodine complex	Sigma-Aldrich	PVP1
29 gauge 0.3 mL insulin syringe	BD	324702
Small Vessel Cauterizer Kit	FST	18000-00
Wound clips	Texas Scientific	205016
AutoClip wound clip applier	BD	427630
AutoClip wound clip remover	BD	427637
Bromodeoxyuridine	Roche	10280879
Heparinized capillary tubes	Fisher	22362566
Microtainer tubes with dipotassium EDTA	BD	365974
20 mL syringe	BD	309661
DPBS	Thermo-Fisher	14190-250
OCT-freezing medium	VWR	25608930
Formalin, Buffered, 10% (Phosphate Buffer)	Fisher	SF100-4
23g needle	Fisher	14-826-6B
FVB/n mouse	Jackson Laboratories	001800