Int J Biol Sci 2010; 6(1):68-79. doi:10.7150/ijbs.6.68 This issue Cite

Research Paper

Keratin promoter based gene manipulation in the murine conducting airway

Stephen P. Malkoski1,3 Corresponding address, Timothy G. Cleaver1, Shi-Long Lu2, Jessyka G. Lighthall*, Xiao-Jing Wang2,3 Corresponding address

1. Division of Pulmonary Sciences and Critical Care Medicine, University of Colorado Denver Health Sciences Center, Aurora CO, USA
2. Department of Otolaryngology, University of Colorado Denver Health Sciences Center, Aurora CO, USA
3. Department of Pathology, University of Colorado Denver Health Sciences Center, Aurora CO, USA
* Current Address: Department of Otolaryngology, Oregon Health & Sciences University, Portland, OR, USA

Citation:
Malkoski SP, Cleaver TG, Lu SL, Lighthall JG, Wang XJ. Keratin promoter based gene manipulation in the murine conducting airway. Int J Biol Sci 2010; 6(1):68-79. doi:10.7150/ijbs.6.68. https://www.ijbs.com/v06p0068.htm
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Abstract

Systems capable of targeting genetic manipulations to keratin-positive airway basal cells are more poorly developed than systems targeting other airway epithelial cell populations and this has likely hindered development of animal models of diseases such as lung squamous cell carcinoma. Although keratin promoter driven-Cre recombinase constructs are potentially useful for targeting these cells, these constructs have substantially higher activity in the skin and oral epithelium than in the airways. We developed a method for delivering RU486, the conditional activator of Cre recombinase progesterone receptor (CrePR) fusion proteins to the lung and then examined the activity of three keratin-driven CrePR constructs in the conducting airways. We also developed a technique for survival bronchioalveolar lavage on non-ventilated animals to examine the effects of the acetone/oil vehicle required to deliver RU486 to the lung. K5CrePR1 and K14CrePR1 constructs differ only in the keratin promoter used to target CrePR1 expression while K5Cre*PR contains a truncated progesterone receptor designed to reduce RU486-independent Cre activity. While all three constructs demonstrate RU486-inducible Cre activity in the conducting airways, both construct activity and tightness of regulation vary considerably. K5Cre*PR is the most tightly regulated Cre driver making it ideal for targeting somatic mutations to the airway epithelia while K5CrePR1 and K14CrePR1 may be better suited to studying diseases of the conducting airways where gene targeting of keratin expressing cells and their derivatives is desired.

Keywords: Keratins, Cre recombinase, basal cells

Introduction

The lung epithelium is comprised of numerous cell types and varies anatomically along the proximal to distal axis. Lung epithelial cells can be derived from different potential progenitor populations during normal development and injury-repair 1-4. Basal cells appear to function as stem cells of the conducting airway by giving rise to other basal cells, Clara cells, and ciliated epithelial cells and by populating the conducting airways during development and after injury 3, 5-7. A variety of systems for targeting Cre recombinase to the lung epithelium have been developed. Constitutive Cre recombinase expression has been targeted to Clara cells via the Clara cell secretory protein (CCSP) promoter, type II alveolar cells via the surfactant protein-C (SP-C) promoter, ciliated epithelial cells via the FoxJ1 promoter 8-11, and less specifically by an adenoviral Cre recombinase vector 12. Similarly, doxycycline-inducible Cre recombinase has been targeted to Clara cells via the CCSP promoter and alveolar type II cells via the SP-C promoter 13, 14. Introduction of oncogenic mutations with these Cre recombinase constructs has usually caused lung adenocarcinoma formation 12, 15, 16 and lung squamous cell carcinomas formation has only rarely been reported 17, potentially because these tumors are derived from keratin-positive airway basal cells not targeted by these approaches.

Both K14CreERT 18 and K5CreERT2 3 express tamoxifen-inducible Cre recombinase-estrogen receptor (ER) fusion proteins under the control of the keratin 14 or keratin 5 promoters and have previously been to lineage label airway basal cells 3, 5, 19. Although systemic tamoxifen treatment permitted temporal control of Cre expression in airway basal cells, it also caused Cre expression in both skin, buccal, and esophageal mucosa in at least one of these studies 5. The lack of a tightly-regulated, basal cell targeting system and an optimized tracheal delivery mechanism of the activator of the Cre-recombinase fusion protein has likely limited the development of mouse models of basal cell specific diseases such as lung squamous cell carcinoma.

Our laboratory previously used a series of keratin-driven, RU486-inducible Cre recombinase-progesterone receptor (PR) fusion proteins for genetic manipulation in the skin and oral epithelium 20, 21. In these systems, keratin promoters are used to restrict the expression of the RU486 inducible Cre recombinase-PR fusion protein; upon treatment with the RU486 activator, the Cre recombinase-PR fusion protein translocates to the nucleus and excises sequences between Lox P sites, facilitating conditional genetic manipulation of target genes 22. We were interested in determining whether these systems could be used to target keratin positive cells of the conducting airways. Because keratins are highly expressed in epidermis and oral epithelium, tracheal delivery of the lipid-soluble RU486 is required to limit gene manipulation to the conducting airway and minimize extrapulmonary Cre activity. In this series of experiments we first established a solvent system for delivering the lipid-soluble RU486 to the lung and then developed a technique for survival bronchioalveolar lavage (BAL) to assess the effects of using an acetone/oil vehicle in the lung. We evaluated the pulmonary and extrapulmonary Cre recombinase activity of three keratin-driven, RU486-inducible, CrePR constructs: K5CrePR1 23 and K14CrePR1 24, which differ in the keratin promoter used to target CrePR1 expression, and K5Cre*PR 20, which differs from K5CrePR1 in that the progesterone element has been truncated to reduce RU486-independent Cre activity. Our experiments show that keratin promoter-directed CrePR expression coupled with direct tracheal delivery of the Cre recombinase activator is a useful way to target airway epithelial cells.

Materials and Methods

Maintenance and use of transgenic mice: Transgenic mice in a C57BL/6 background were maintained in specific pathogen free rooms in accordance with Oregon Health & Sciences University or University of Colorado Denver policies on animal use and care; all procedures were approved by Institutional Animal Care and Use Committees. Keratin 5 CrePR1 (K5CrePR1) and Keratin 14 CrePR1 (K14CrePR1) mice express a truncated, RU486-inducible, progesterone receptor-Cre recombinase fusion protein under the control of a keratin 5 or keratin 14 promoter 23, 24. The Keratin 5 Cre*PR (K5Cre*PR) construct has an additional 16 amino acid deletion of the progesterone receptor (PR) designed to reduce RU486-independent Cre recombinase activity 20, 25. Rosa26 reporter mice contain a lox-neomycin-lox sequence between a constitutive promoter and a β-galactosidase (β-gal) reporter 26. Bigenic reporter mice were created by crossing K5CrePR1, K14CrePR1, K5Cre*PR mice with Rosa26 reporter mice to create mice heterozygous for both genes (Figure 1A). For each CrePR construct, one founder line that previously exhibited robust Cre activity in either the skin or oral mucosa was used for tracheal delivery experiments.

Experiments were performed on 3-4 week old mice and experimental groups contained at least 3 mice from multiple litters (individual experimental numbers are described in figure legends). K5CrePR1.Rosa26 mice were treated with 100μg of tracheal RU486 and β-gal activity assessed 7 days later. K14CrePR.Rosa26 mice were treated with two 500μg doses of tracheal RU486 given 5d apart and β-gal activity evaluated 7 days later after the last RU486 dose. K5Cre*PR.Rosa26 mice were treated with two 500μg tracheal RU486 doses given 5d apart then sacrificed either 7 days or 24 weeks after the last RU486 dose. Both male and female mice were used in all experiments; no gender differences were observed.

 Figure 1 

(A) Keratin CrePR mice express a Cre recombinaseprogesterone receptor (PR) fusion protein whose expression is restricted by a K5 or K14 promoter. CrePR is inducible by the progesterone antagonist RU486 but not by endogenous progesterone. Upon induction with RU486, CrePR translocates into the nucleus and excises DNA sequences flanked by Lox P sites. Rosa26 reporter mice contain a lox P-neomycin-lox P sequence between a constitutive promoter and a β-gal reporter hence after Cre recombinase-mediated excision of the neomycin cassette β-gal is constitutively expressed and can be used to monitor Cre recombinase activity. (B) Immunofluoresence for K5/K14 positive basal cells in the human and mouse trachea demonstrates the simpler conducting airway epithelium in the mouse. Minimal background immunostaining was observed when sections were incubated without primary antibody (not shown). The immunostaining pattern is consistent with marking K5/K14 positive basal cells. In the human trachea there are 23.4 ± 1.4 (mean ± SEM) K5 positive cells/100 μm epithelium and 5.6 ± 0.9 K14 positive cells/100 μm epithelium (p<0.05 for K5 vs. K14 positive). In the mouse, there are 13.6 ± 2.6 K5 positive cells/100 μm epithelium and 1.9 ± 0.9 K14 positive cells/100 μm epithelium; in the axial bronchus there are 7.5 ± 2.1 K5 positive cells/100 μm epithelium and 0.25 ± 0.2 K14 positive cells/100 μm epithelium (p<0.05 for K5 positive vs. K14 positive in both murine trachea and axial bronchus).

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Tracheal intubation, drug delivery, and bronchioalveolar lavage (BAL): Tracheal intubation was performed as previously described 27 with minor modifications. Briefly, mice were anesthetized with mouse cocktail (30mg/ml ketamine; 3mg/ml xylazine; 0.6mg/ml acepromazine; 70μl/20g mouse i.p.) or 2-3% isoflurane and placed at a 60° angle suspended by the top incisors. The trachea was transilluminated at the thoracic inlet and a bent chemical spatula used as a laryngoscope. Vocal cords were directly visualized and a 20-gauge angiocath placed via a Seldinger technique. Correct tube positioning was confirmed by observing abdominal breathing with brief occlusion of the tube. RU486 (Biomol, Plymouth Meeting, PA) dissolved in various solvents was instilled into the trachea as detailed in Table 1. For 50% organic solvent/saline trials 5 mice/group were used; for acetone/sesame oil trials, 9-11 mice/group were used. Dye delivery to evaluate anatomic precision of tracheal delivery was performed as follows. First, 10μl of 0.01% Evans blue dye in 10% acetone/90% sesame oil solvent was drawn up into a previously calibrated length of PE10 tubing affixed to a blunted 25-gauge needle and a 1mL syringe. After tracheal intubation, PE10 tubing was passed though the tracheal angiocath until slight resistance was met; dye was then instilled over 2-3 seconds. Animals were immediately extubated. Mice were sacrificed within 1 hour to evaluate dye distribution in the in the lungs.

Survival bronchioalveolar lavage (BAL) was performed using isoflurane anesthesia and a 4cm length of PE20 tubing attached to a 1mL syringe containing 200μl of normal saline. After tracheal intubation, PE20 tubing was passed through the catheter until slight resistance was encountered. Sterile normal saline (200μl) was instilled over 5 seconds and immediately withdrawn and placed on ice. Following BAL, mice were extubated and returned to their cages to recover. BAL fluid was cytospun onto slides (5min at 500rpm) then stained with either Diff Quik (Fisher Scientific, Pittsburg, PA) or Oil Red O (Sigma, St Louis, MO). Differential cell counts were determined by morphological criteria and differences between groups compared by unpaired t-tests.

Immunofluoresence (IF) and Immunohistochemistry (IHC): IF and IHC were performed as previously described 21. After heat-mediated antigen retrieval in 10mM citrate for 10min, sections were incubated overnight at 4°C with antibodies against Keratin 5 (1:500 Abcam, Cambridge, MA), K14 (1:1000, Abcam), p63 (1:50 Santa Cruz Biotechnology, Santa Cruz, CA), or CCSP (1:2000 Upstate, Billerica, MA); antigen was detected by incubation with species-appropriate, fluorochrome- conjugated secondary antibody (1:100 Invitrogen, Carlsbad, CA) or biotinylated secondary antibody (1:100, Vector Laboratories, Burlingame, CA).

β-gal staining: β-gal activity was evaluated as previously described 5. After euthanasia, whole organs were removed and fixed for 20 min in 4% parafomaldehyde at room temperature, rinsed in PBS, then incubated at 37°C for 4-16h in X-gal staining solution [2mM MgCl2, 5mM K4Fe(CN)6, 5mM K3Fe(CN)6, 0.02% NP40, 0.01% sodium deoxycholate, 1mg/ml 5-bromo-4-chloro-3-indolyl-β-D-galactopy­ranoside (X-gal)], then postfixed in 4% paraformaldehyde overnight at 4°C. β-gal activity in whole organs was photographed through a Nikon SMZ1000 dissecting microscope with a Nikon DS Ri1 camera using Nikon Elements software. β-gal stained organs were paraffin embedded, sectioned, and counterstained with nuclear fast red or with immunohistochemistry as described above. The recombination frequency was determined by counting the number of β-gal positive cell per 100 μm tracheal epithelium in at least 3 separate tracheal sections.

Human tracheal samples: Normal human tracheal sections from lung transplant donors were provided by Dr. David Jacoby (Oregon Health & Sciences University, Portland, OR) with approval of the Institutional Review Board. Three human tracheal samples were evaluated.

Results

Keratin expression in murine conducting airways: In human airways, the number of keratin positive basal cells is ~30% in the large (>4mm) airways but falls to 6% in airways <0.5mm 28. Similarly, basal cells (identified by histology) comprise ~18% of airway epithelial cells in the mouse trachea but <3% of airway epithelial cells in the axial bronchus and distal airway 29. We confirmed a similar distribution of K5 positive cells in the human trachea, mouse trachea, and mouse axial bronchus. Interestingly, K14 expression appeared restricted to a subset of K5 positive cells in all three conducting airway epithelia (Figure 1B). Compared to the human trachea, in the mouse trachea, K5 positive basal cells are less numerous and restricted to a single cell layer. Though clearly more numerous in the trachea, basal cells (identified by K5 staining) are still detectable in the lobar bronchus (Figure 1B). These observations support the hypothesis that keratin promoters can target gene manipulation to the murine conducting airways.

Optimization of tracheal RU486 delivery: Because keratins are expressed in many epithelial tissues including the skin, oral mucosa, and urogential mucosa, targeting keratin positive airway cells without targeting keratin positive cells in other epithelial layers requires both tracheal delivery of the conditional gene activator and a system with minimal activator-independent Cre recombinase activity. Because RU486, the conditional activator of the truncated progesterone receptor-Cre recombinase, has minimal aqueous solubility, we investigated alternative solvents for tracheal RU486 delivery (Table 1). The goal of these experiments was to determine whether animals would tolerate tracheal delivery of the 50% organic solvent mixtures necessary to dissolve RU486. While tracheal instillation of 50μl normal saline is well tolerated, the organic solvents required to dissolve RU486 were associated with unacceptably high mortality upon tracheal instillation. In addition, these solvent combinations were only capable of delivering 10μg of RU486. When RU486 was dissolved in acetone (at 100μg/μl) then diluted 1:10 with sesame oil, 10μl of 10% acetone/90% sesame oil was well tolerated and 100μg RU486 could be delivered with a 11% mortality; when the volume was increased to 20μl, mortality increased to 22%. Because respiratory depression secondary to ketamine/xylazine anasthesia was though to contribute to mortality after tracheal instillation of a viscous vehicle, we tested whether a shorter acting inhalational anesthetic would reduce procedural mortality and found that with isoflurane anesthesia, a higher concentration of acetone (20%) and larger volume (25μl) facilitated the tracheal delivery of up to 500μg of RU486 without appreciable mortality.

 Table 1 

Mortality of various solvents evaluated for tracheal RU486 delivery Mortality is expressed as both a percentage and raw number. For all vehicle combinations except 20% acetone/80% sesame oil, ketamine anesthesia was used. With 50% DMSO/50% saline and 50% acetone/50% saline, death occurred immediately upon instillation while with 50% ethanol/50% saline, death occurred 3-5 days later. With the acetone/oil vehicles, all observed mortality occurred with instillation.

VehicleVolumeMortality RU486
Normal saline50μl0% (0/5)0μg
50% DMSO/50% saline10μl100% (5/5)10μg
50% acetone/ 50% saline10μl100% (5/5)10μg
50% ethanol/50% saline10μl80% (4/5)10μg
10% acetone/90% oil10μl11% (1/9)100μg
10% acetone/90% oil20μl22% (2/9)200μg
20% acetone/80% oil (isoflurane anesthesia)25μl0% (0/11)500μg

To assess the anatomic precision of tracheal delivery, we instilled Evans blue dye into either the trachea (Figure 2A) or the right main bronchus (Figure 2B) as described in the Methods. With tracheal dye instillation, minimal staining was observed in the esophagus while marked staining of the trachea and lung occurred (Figure 2A), demonstrating that this technique does not result in significant inadvertent exposure of other keratin expressing tissues (e.g., the oropharynx). The ability to deliver this vehicle almost exclusively to one lung (Figure 2B) shows the feasibility of unilaterally targeting lung cancer inducing genetic alterations to either prevent premature death from tracheal obstruction or to allow additional time for lesions to progress to full malignancy or metastasize.

Clearance of Lipid Laden Macrophages After Tracheal Delivery of Sesame Oil: One concern regarding the use of sesame oil to deliver RU486 to the lungs is the development of a lipoid pneumonia characterized by an abundance of lipid-laden macrophages (LLMs), as occurs with chronic lipid aspiration in humans 30. To examine this possibility we evaluated LLM clearance from the BAL fluid using survival BAL as described in the Methods. Using isoflurane anesthesia, survival BAL can be performed on non-ventilated mice with a mortality of <8% and a return of approximately 50% of the lavage fluid volume. Mice appeared normal within hours after survival lavage, without evidence of respiratory distress, tachypnea, or huddled posture. All procedural mortality was immediate suggesting asphyxia as the cause of death; no delayed mortality consistent with pneumonia was observed. On untreated animals survival BAL specimens are >95% macrophages, however, 3d after tracheal instillation of 20μl of 20% acetone/80% sesame oil, 50% of cells recovered by BAL are LLM, while 45d after instillation, 8% of cells recovered by BAL are LLM (Figure 2C). Tracheal instillation of acetone/sesame oil causes a modest inflammatory response with neutrophils comprising 26% of BAL cells 3d after tracheal instillation; however, this inflammation resolves almost completely 45d post instillation. Despite the short-term inflammatory response demonstrated by BAL, there was no obvious inflammation or morphological abnormalities in either the conducting airways or lung parenchyma at 5 days, 5 weeks, or 5 months after instillation of RU486 in acetone/sesame oil vehicle (Supplemental Figure S1). In addition to describing a technique for repeatedly sampling the lower airways in non-ventilated mice, these observations document LLM clearance after instillation of a lipid-based RU486 carrier.

Cre recombinase activity in K5CrePR1.Rosa26 mice: We initially examined K5CrePR1 activity in the trachea because this construct exhibited the most robust activity in both skin and oral mucosa 20, 21, 23. RU486 (100μg in acetone/sesame oil) was delivered to the trachea then Cre activity was detected by β-gal staining 7 days later. Tracheal dosing and timing was chosen based on doses previously used for gene manipulation in other keratin expressing epithelial tissues 20, 21, 23. Although vehicle treated K5CrePR1.Rosa26 mice exhibited a modest amount of RU486-independent activity (Figure 3A, middle panels), RU486 caused a significant induction in tracheal Cre activity as evidenced by the extensive β-gal staining in both whole mount and histology sections (Figure 3A, right panels). To characterize the airway cells targeted by K5CrePR1, tracheal sections from RU486 treated K5CrePR1.Rosa26 mice were immunostained for the basal cell markers, K5 and p63, and the Clara cell marker, CCSP. We found that β-gal staining co-localized with K5 and p63 immunostaining confirming that airway basal cells are targeted by K5CrePR1. That β-gal staining also co-localized with CCSP positive cells suggests either that previously targeted basal cells have differentiated into Clara cells 5, 19 or that the K5CrePR1 construct also targets Clara cells.

 Figure 2 

(A) Excised heartlung block after tracheal instillation of 10μl 0.01% Evans blue dye in 10% acetone/90% sesame oil showing staining in the trachea and lung but not in the esophagus. (B) Evans blue dye instillation to the right lung was performed as described in the methods. (C) Recovery of LLM by survival BAL after tracheal instillation of acetone/sesame oil. Untreated 8-12 week old animals (n=12) underwent BAL with 200μl normal saline as described in Methods. Approximately 95% of recovered cells were macrophages. A separate group of mice (n=15) was treated with 20μl of 20% acetone/80% sesame oil on day 0 then underwent survival BAL on either day 3, 21, or 45 (n=5 for each time point). Three days after treatment there was marked increase in both LLM and neutrophils (bottom left), however, these changes largely resolved by day 45. * p<0.05 vs. untreated control for all cell types; **p<0.05 vs. days 3 and 21 for all cell types.

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 Figure 3 

Cre activity after tracheal RU486 in K5CrePR1Rosa26 mice. (A) K5CrePR1.Rosa26 mice were treated with 100μg tracheal RU486 and β-gal activity assessed 7d later. No β-gal staining was observed in Cre negative monogenic littermates while RU486-inducible Cre activity was seen in K5CrePR1.Rosa26 animals. Representative images are shown; 3-4 mice/group were analyzed for β-gal expression. The dashed line delineates the epithelial basement membrane; the scale bar represents 100μm. Untreated K5CrePR1.Rosa26 mice had 5.3 ± 1.0 (mean ± SEM) recombinant cells/100μm tracheal epithelium while RU486-treated mice had 14.5 ± 4.2 recombinant cells/100μm tracheal epithelium (p=0.05). (B) Co-localization of β-gal staining with K5, p63, and CCSP expression in K5CrePR1.Rosa26 mice treated with tracheal RU486. Arrows indicate co-localization of β-gal and immunohistochemical staining in basal cells (K5+ and p63+) and Clara cells (CCSP+).

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Inducible Cre recombinase activity in K14CrePR1.Rosa26 mice: While K5CrePR1 can be activated in the trachea, as animals age, substantial RU486-independent activity occurs in many keratin expressing tissues (not shown), however this activity is typically less than RU486-induced activity 21, 31. We evaluated whether K14CrePR1 could direct Cre activity to the trachea and whether K14CrePR1 also exhibited RU486-independent Cre activity. K14CrePR1.Rosa26 mice were treated with tracheal RU486 (two 500μg doses given 5d apart) and sacrificed 7d after the last RU486 dose to evaluate β-gal activity. A higher RU486 dose was used in experiments with both K14CrePR and K5Cre*PR as lower doses appeared relatively ineffective in inducing Cre activity in pilot experiments (not shown). The RU486-independent activity of K14CrePR1 was markedly less than that of K5CrePR, and although β-gal positive cells could be seen on vehicle-treated whole mount tracheal sections, it was difficult to detect these cells in histology sections. After RU486 treatment, however, discrete areas of β-gal staining were clearly seen in the whole mount trachea and were more apparent when the trachea was opened longitudinally (Figure 4A). In addition, distinct β-gal staining was occasionally seen in the lung parenchyma (Figure 4A, right); consistent with either the presence of rare basal cells in the more distal airways or sporadic targeting of more distal Clara cells. Immunostaining for K5, p63, and CCSP again colocalized with β-gal staining (Figure 4B) suggesting that K14CrePR1 targets basal cells and their progeny. Compared to K5CrePR1, K14CrePR1 exhibits both less RU486-independent and RU486-induced Cre activity, perhaps because K14 is only expressed in a subset of K5 positive basal cells (see Figure 1B).

K5Cre*PR is tightly regulated with inducible and persistent Cre activity: The K5Cre*PR construct is analogous to K5CrePR1 except for a 16 amino acid deletion of the truncated progesterone receptor designed to reduce RU486-independent Cre recombinase activity 25. This construct has been used in mouse models of both skin and oral cancer 21, 32. We wanted to determine whether this construct would be active in the conducting airways and whether it would exhibit less RU486-independent activity than K5CrePR1 or K14CrePR1. K5Cre*PR.Rosa26 mice were treated with tracheal RU486 (two 500μg doses 5d apart) then sacrificed 7d after the last RU486 dose. We observed minimal RU486-independent activity in the airways (Figure 5A) or in other keratin expressing tissues (not shown); however, RU486 was still capable of inducing tracheal Cre activity (Figure 5A). Although K5Cre*PR has less tracheal Cre activity than K5CrePR1 or K14CrePR1, Cre activity still localized to K5/p63 positive basal cells and Clara cells (Figure 5B). Because K5Cre*PR was the most tightly regulated construct tested, we assessed whether Cre-mediated gene recombination persisted after RU486 treatment and found increased β-gal activity in K5Cre*PR.Rosa26 animals 24 weeks after tracheal RU486 treatment compared to either vehicle treated animals or animals assessed 7d after treatment (Figure 5C). Again, β-gal staining colocalized with K5, p63, and CCSP immunostaining, however, at this time point a larger fraction of tracheal epithelial cells had been labeled, consistent with the hypothesis that recombination initially occurred in a basal cell progenitor.

 Figure 4 

Cre recombinase activity in K14CrePR1Rosa26 mice. Mice were treated with 500μg of tracheal RU486 on days 1 and 5 and then assessed for β-gal activity 7d after the last RU486 dose. (A) Cre activity was induced in the trachea and was localized to discrete areas in the tracheal epithelium, however, β-gal staining was also occasionally observed in the lung parenchyma, consistent with rare basal cells in more distal airways. Representative images are shown; 3-8 mice per group were analyzed for β-gal expression. (B) Immunohistochemistry for K5, p63, and CCSP colocalizes with β-gal staining in K14CrePR1.Rosa26 mice treated with tracheal RU486. The scale bar represents 50μm; arrows indicate co-localization of β-gal with K5, p63, and CCSP immunohistochemical staining; 1.3 ± 0.6 recombinant cells/100μm tracheal epithelium were observed in RU486 treated animals compared to 0.1 ± 0.07 recombinant cells/100μm tracheal epithelium in vehicle treated animals (p<0.05).

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 Figure 5 

Inducible and persistent Cre recombinase activity in K5Cre*PRRosa26 mice after tracheal RU486. (A) In mice treated with 500μg of tracheal RU486 on days 1 and 5 and assessed for β-gal activity 7d later, discrete areas of β-gal activity were seen in the trachea. β-gal staining was not observed in the tongue or esophagus of RU486-treated animals (not shown) or in vehicle treated animals. Representative images are shown; 5-10 mice per group were analyzed. (B) β-gal activity colocalized with K5, p63, and CCSP immunostaining in the trachea of RU486-treated K5Cre*PR.Rosa26 mice. The scale bar represents 50μm; arrows indicate co-localization of β-gal and immunohistochemical staining; 0.3 ± 0.16 recombinant cells/100μm tracheal epithelium were observed in RU486 treated mice; recombinant cells could not be found in the tracheal epithelium of vehicle treated animals. (C) Persistent tracheal Cre recombinase activity in K5Cre*PR.Rosa26 mice 24 weeks after tracheal RU486. Although β-gal staining was weaker compared to earlier time points, it still colocalized with K5, p63, and CCSP staining and was not detected in vehicle-treated tissues (top panel). The scale bar represents 50μm; 17.5 ± 0.8 recombinant cells/100μm tracheal epithelium were observed (p<0.05 vs. 7d after RU486).

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Discussion

This study describes how a series of keratin-driven, conditionally activated Cre recombinase constructs in combination with tracheal delivery of the Cre inducer can be used for gene manipulation in murine conducting airway. While all three keratin CrePR constructs target the conducting airway epithelium, there are important differences that will influence use of these constructs. K5CrePR1 provides robust Cre activity and genetic recombination in most of epithelial cells of the murine trachea but has substantial ligand-independent activity in the trachea as well as in the skin and oral mucosa that could limit the utility of this construct if genetic recombination outside the lung is problematic. Nonetheless, K5CrePR1 may be ideal if genetic recombination is required in a high proportion of tracheal epithelial cells and extrapulmonary Cre activity is unimportant, for example in producing a culture of primary tracheal epithelial cells with a specific gene manipulation for in vitro studies or assessing susceptibility of the conducting airway epithelium to carcinogens after deletion of a tumor suppressor. In this study, we did not rigorously determine which tracheal epithelial cells express K5CrePR1 in the absence of induction or whether K5CrePR driven recombination persists over months. K5CrePR1 causes genetic recombination in a higher proportion of the conducting airway epithelium than the induced K14CreER construct 5, 19 and appears to target a similar proportion of tracheal epithelial cells as the induced K5CreERT2 construct 3.

K14CrePR1 has less RU486-independent activity than K5CrePR1 and is inducible in a fraction of K5 positive basal cells by tracheal RU486. While K14CrePR1 is less active than K5CrePR1, this may be reflective of fewer K14 positive than K5 positive tracheal basal cells, however, the tissue distribution and tracheal activity of K14 directed Cre activity is similar to what was previously reported with K14CreERT after induction with systemic tamoxifen 5, 18, 19 and is consistent with the K14 expression observed in the murine trachea. When K14CreERT was used for lineage tracing basal airway cells, systemic tamoxifen was used for induction and ligand-independent Cre activity in the conducting airways was not reported 5, 19, making it difficult to directly compare K14CrePR1 and K14CreERT. In any case, K14CrePR1 could potentially be used for evaluating lineage relationships between K14 positive tracheal cells and other cell types but would not be effective if experimental design required comprehensive alteration of gene expression in the entire K5 positive basal cell population. Our study suggests it may be possible to use a similar lipid delivery system for the 4-hydroxytamoxifen inducer of K14CreERT or K5CreERT2 to achieve airway basal cell gene manipulation while minimizing Cre activity in other tissues.

Although overall inducible Cre activity of K5Cre*PR is less than that of K5CrePR1 or K14CrePR1, K5Cre*PR displays almost no ligand-independent Cre activity in the trachea or other keratin positive tissues (not shown). Induction with tracheal RU486 results in Cre activity in tracheal basal cells and Clara cells that increases with time and is consistent with targeting of basal cells that then give rise to additional basal cells, Clara cells, and ciliated epithelial cells as previously reported with the K5CreERT2 construct 3. While K5Cre*PR would not be a good choice if experimental design required gene manipulation in the entire basal cell population, that K5Cre*PR is more tightly regulated makes it an attractive construct for use in cancer models where targeting of sporadic mutations would more closely mimic the somatic mutations leading to the development of human cancer. Our data also suggests that extra-pulmonary recombination can be minimized by tracheal RU486 delivery. Though this approach has not yet been reported in the lung, K5Cre*PR has been used to generate tumors in both the skin and oral epithelium via knock-in of K-rasG12D 21, 32.

Presumably because of concerns regarding lipoid pneumonia or inflammation, reports of oil-based vehicles for lung delivery are limited. Although steroids are routinely delivered to the airways in clinical practice, this is typically done using an aerosol, an approach that is challenging in the experimental setting with very small quantities of material and when wanting to avoid delivery to the oropharynx or nasopharynx. One report demonstrated that a mixture of ethyl acetate/olive oil failed to deliver toluene diisocyanate (TDI) to the lung when administered by nasal inhalation 33, while another report described repeated tracheal instillations with TDI in olive oil 34. Although the second report demonstrated an increase in BAL eosinophils, inflammation, and goblet cell hyperplasia with TDI-olive oil instillation, the presence of LLM was not described 34. We show that an acetone/sesame oil mixture can safely deliver RU486 to the mouse lung but causes a short-term inflammatory response comprised of neutrophils and LLM. Despite the inflammatory response demonstrated by survival BAL, there is minimal evidence of inflammation in the conducting airways or lung parenchyma (Supplemental Figure S1). While it cannot be excluded that inflammation contributes to Cre activation, Cre activity in the airways of vehicle treated and untreated K14CrePR1.Rosa26 mice was similar (not shown) and there is minimal Cre activity in vehicle treated K5Cre*PR.Rosa26 mice. Taken together, our data show that a single pulmonary dose of lipid/organic solvent is better tolerated than anticipated.

In the process of evaluating the response to tracheal instillation of potential RU486 vehicles, we developed a simple but potentially useful technique for performing survival BAL on non-ventilated mice. Although repeated BAL of individual ventilated mice has been reported 35, the widespread use of this technique has likely been limited by the requirement for mechanical ventilation. Although the amounts of instilled and recovered lavage fluid are reduced compared to mechanically ventilated mice (200μl instilled and ~100μl recovered vs. 600μl instilled and ~420μl recovered), our technique is simple and permits repeated sampling of individual animals over time, potentially reducing the number of animals required for a given study, and allowing each animal to serve as its own control. In addition, although we report an overall mortality of 8% for this technique, the mortality fell with increasing operator experience. This approach could be particularly useful for studies examining recovery of infectious agents or BAL cellular profiles in response to various stimuli even though the amount of recovered BAL fluid may limit some downstream applications.

In summary we developed a method for delivering lipid soluble Cre activators to the lung that is safe and effective and can be used to minimize extra-pulmonary Cre recombinase activity when using keratin driven Cre constructs or other inducible Cre constructs targeted by broadly expressed promoters. These approaches should facilitate the modeling of diseases thought to arise from airway basal cells such as lung squamous cell carcinoma.

 Supplemental Figure S1 

Hematoxylin and eosin stained sections of the trachea axial bronchus and lung parenchyma 5 days, 5 weeks, and 5 months after instillation of 500μg RU486 in 20μl of 10% acetone/90% sesame oil showing no obvious inflammation or morphological abnormality. The scale bar represents 100μm.

Int J Biol Sci Image

Acknowledgements

We thank Dr. David Jacoby for providing human tracheal sections. This work was supported by the NIH/NCI (F32 CA119467 and K08 CA131483 to S.P.M.) and NIH/NIDCR (R01 DE015953 to X.J.W.). S.P.M. was also supported by T32-CA 106195 (“Training in Skin Pathobiology”) and the Oregon Medical Research Foundation.

Conflicts of interest

The authors report no conflict of interest. The authors alone are responsible for the content and writing of this manuscript.

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Author contact

Corresponding address Correspondence to: Xiao-Jing Wang, MD, PhD, Departments of Pathology, Dermatology and Otolaryngology, 12800 E. 19th Avenue, Research 1 North, Room 5128, Box 8104 Aurora, CO 80045. Phone: 303-724-3001 Fax: 303-724-4730 Email: XJ.Wangedu. Or Stephen Malkoski, MD, PhD, Division of Pulmonary Sciences and Critical Care Medicine and Pathology,12800 E. 19th Avenue, Research 2, C272, Aurora, CO 80045. Phone: 303-724-6058 Fax: 303-724-4730 Email: Stephen.Malkoskiedu


Received 2009-12-10
Accepted 2010-1-15
Published 2010-1-20


Citation styles

APA
Malkoski, S.P., Cleaver, T.G., Lu, S.L., Lighthall, J.G., Wang, X.J. (2010). Keratin promoter based gene manipulation in the murine conducting airway. International Journal of Biological Sciences, 6(1), 68-79. https://doi.org/10.7150/ijbs.6.68.

ACS
Malkoski, S.P.; Cleaver, T.G.; Lu, S.L.; Lighthall, J.G.; Wang, X.J. Keratin promoter based gene manipulation in the murine conducting airway. Int. J. Biol. Sci. 2010, 6 (1), 68-79. DOI: 10.7150/ijbs.6.68.

NLM
Malkoski SP, Cleaver TG, Lu SL, Lighthall JG, Wang XJ. Keratin promoter based gene manipulation in the murine conducting airway. Int J Biol Sci 2010; 6(1):68-79. doi:10.7150/ijbs.6.68. https://www.ijbs.com/v06p0068.htm

CSE
Malkoski SP, Cleaver TG, Lu SL, Lighthall JG, Wang XJ. 2010. Keratin promoter based gene manipulation in the murine conducting airway. Int J Biol Sci. 6(1):68-79.

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