Background
Pulmonary surfactant, a complex mixture of lipids and proteins, is produced and secreted by alveolar type II cells [
1]. Approximately 10% of the surfactant is formed by proteins, which contain the hydrophilic surfactant proteins A and D (SP-A and SP-D, respectively) as well as the hydrophobic surfactant proteins B and C (SP-B and SP-C, respectively) [
2]. Human SP-A genes are located on chromosome 10q22-q23 [
3]. Two functional genes, SP-A1 and SP-A2, which share 96% and 97% similarities in amino acid and nucleotide sequences, respectively, encode SP-A [
4,
5]. SP-A also has characteristic structures similar to those of the C-type lectin superfamily, which forms a flower bouquet structure composed of six trimeric subunits, each of which consists of 26 kDa to 35 kDa monomers [
1,
6]. Alveolar type II and Clara cells in the lungs are the primary cells that secrete SP-A, which plays a role in preventing the pulmonary alveoli from collapsing after expiration [
7]. The expression of SP-A, which is not restricted to the respiratory system, was also detected in gastric, intestinal [
8], vaginal [
9], skin [
10], middle ear [
11], and Eustachian tube [
12] epithelia. Similar to the lungs, the kidneys are derived from the endoderm and are exposed to external pathogens. Thus, the kidney is likely one of the sites where SP-A can be expressed.
SP-A participates in the pathophysiological and physiological regulation of the inflammatory process in the lungs [
13]. SP-A can bind to several bacterial, viral, and fungal pathogens, thereby resulting in growth inhibition and opsonisation of these pathogens [
14]. SP-A knockout mice were reported to exhibit increased levels of proinflammatory cytokines and decreased ability of phagocytosis by alveolar macrophages [
15]. George et al. [
16] reported that the complete SP-A gene expression in the lungs is increased after repeated exposure to an inhaled endotoxin. Lipopolysaccharide (LPS), a major component of the outer membrane of Gram-negative bacteria, induces various inflammatory mediators, including tumour necrosis factor, interleukin-1, and interferon [
17]. A recent study has also shown that LPS selectively induces SP-A gene expression possibly through TLR2-mediated activation of c-Jun in human alveolar epithelial A549 cells [
18]. However, the effect of LPS on the regulation of SP-A expression in human tubular epithelial-like HK-2 cells is not well known.
In the present study, we determined whether SP-A1 and SP-A2 mRNA and proteins are expressed in human renal tissues and HK-2 cells. We also evaluated the effects of LPS on the regulation of SP-A subtype expressions in HK-2 cells.
Materials and methods
Materials
Human renal tissue samples obtained from 10 patients (six males and four females, 58 ± 12 years old) who underwent operations for renal cancer were used in the present study. Furthermore, lung tissue samples were obtained from five patients who underwent operations for lung cancer (two females and three males, 62 ± 5 years old). The experimental procedure was carried out according to the protocol approved by the Human Ethics Committee of the Renmin Hospital of Wuhan University in China.
Cell cultures
Renal tubular epithelial cells (HK-2, a proximal tubular cell line derived from normal kidney; purchased from ATCC, CRL-2190) were cultured at 37°C in a humidified atmosphere of 5% CO2 and then treated with Dulbecco’s modified Eagle’s medium (DMEM, Hyclone Pierce, USA) in a mixture of 10% foetal bovine serum (Invitrogen, USA) and 1% ampicillin. The culture medium was changed every 2 d until the cells reached 70% to 80% confluency, at which point they were dissociated with 0.25% trypsin/EDTA. Subsequently, the cells were incubated for 24 and 72 h to determine mRNA and protein expressions, respectively.
Immunohistochemical experiment
Human renal tissues were embedded in paraffin (4 μm thick) and then immunohistochemically examined using a SP-A polyclonal antibody (supported by Prof. Guirong Wang [
19]). After the tissue sections were washed and incubated with 5% H
2O
2 in methanol for 30 min at room temperature to inhibit endogenous peroxidase activity, they were incubated with a primary antibody (rabbit anti-human polyclonal SP-A at a dilution of 1:150) at 4°C overnight. The sections were washed in phosphate-buffered saline (PBS) repeatedly and then incubated with an anti-rabbit secondary antibody conjugated with horseradish peroxidase. Negative controls were stained with PBS instead of the primary antibody. Slides were rinsed in PBS and then incubated in diaminobenzidine chromogen (Solarbio, China). Colour development was observed under a microscope. The slides were counterstained with haematoxylin to determine the presence of nuclei.
RT-PCR
Normal human renal tissues and cultured HK-2 cells were used for RT-PCR analysis of SP-A and GADPH mRNA, and alveolar tissues were used as positive controls. An oligonucleotide dT primer and primer pairs of the target and control genes, respectively, for RT-PCR were purchased from Invitrogen Corporation (Table
1). Total RNA was extracted from each sample with Trizol (Invitrogen, USA) following the manufacturer’s instructions. Total RNA (1 μg) extracted from the tissue was used for the RT reaction (Takara, China), and then 1 μL of cDNA was used for amplification at a final volume of 20 μL according to the supplier’s protocol (Fermentas, Germany). Each PCR product (6 μL) was subjected to electrophoresis on 2% agarose gel.
Table 1
Primers used for amplification of SP-A1, SP-A2 and SP-A
SP-A | F-GAAGGACGTTTGTGTTGGAA | 56.1 | 35 | 439 |
commom to SP-A1 and A2 | R-TGGATTCCTTGGGACAGCAA | | | |
SP-A | F-CACTTTTGATGCCATTCAGGAG | 56.3 | 35 | 295 |
commom to SP-A1 and A2 | R- GGTCAGTCGGGAGTACAGGC | | | |
SP-A1 | F-TGGGCAAGGTAATCAGTG | 49.1 | 33 | 365 |
| R-GTCCAGGAAGATGGGTTT | | | |
SP-A2 | F-TATTGACCGAGCACATACC | 49.3 | 33 | 212 |
| R-GTCCAGGAAGATGGGTTT | | | |
GADPH | F-TCCCTGGAGAAGAGCTACGA | 53.5 | 30 | 200 |
| R-TCGTCATACTCCTGCTTGCT | | | |
Detection of the gene expressions of SP-A1 and SP-A2 mRNA
Approximately 10 μL of the PCR product (a primer pair common to SP-A1 and SP-A2, 439 bp) was digested using 2 μL of the restriction enzyme Apa I (Toyobo, Japan), 2 μL of 10× buffer B, and 18 μL of double-distilled water at 37°C for 12 h. The treated PCR product (8 μL) was then electrophoresed on 2% agarose gel.
Another PCR product (a primer pair common to SP-A1 and SP-A2; 295 bp) was subjected to electrophoresis on 2% agarose gel and then purified using a TIANgel Midi purification kit (TianGen, China) according to the manufacturer’s instructions. Sequencing was then directly performed using an ABI 3730xl 96-capillary DNA analyser.
Western blot
Proteins from human tissues (kidneys and lungs) and HK-2 cells were extracted using RIPA lysate [150 mM sodium chloride, 1.0% Triton X-100, 0.5% sodium deoxycholate, 0.1% sodium dodecyl sulphate (SDS), and 50 mM Tris at pH 8.0]. The total protein concentrations were determined using the bicinchoninic acid protein assay (Hyclone Pierce). Total protein (50 μg) was resolved by reducing 12% SDS-polyacrylamide gel electrophoresis and then transferred electrophoretically at 60 mA onto nitrocellulose membranes at 4°C overnight (Bio-Rad, USA). After the samples were blocked in 5% non-fat milk in Tris-buffered saline, immunoblotting was detected using a primary antibody against SP-A(rabbit anti-human polyclonal SP-A at a dilution of 1:150) and a anti-rabbit secondary antibody conjugated with horseradish peroxidase. Cellular β-actin protein was immunodetected using a human monoclonal antibody against human β-actin (Sigma) as the internal standard. Immunoproducts were detected using enhanced chemiluminescence peroxidase detection reagents (Amersham, Sweden).
LPS-induced expressions of SP-A1 and SP-A2 mRNA and protein in HK-2 cells
HK-2 cells were incubated with various concentrations (0, 0.1, 1, 2, 5, and 10 μg/mL) of LPS from Escherichia coli 0111:B4 (Sigma) for 8 h and then with 5 μg/mL of LPS at different time points (0, 2, 4, 8, 16, and 24 h). The cells were collected to detect the expressions of SP-A1 and SP-A2 mRNA and SP-A protein as described above.
Statistics
Data were expressed as mean ± SEM. Results were analysed using one-way ANOVA with SPSS 13.0 software. P < 0.05 was considered to indicate statistical significance.
Discussion
The present study demonstrated the expression and localisation of SP-A within the renal tissue. LPS selectively induced the expressions of SP-A1 and SP-A2 mRNA and protein in human tubular epithelial-like HK-2 cells in time- and dose-dependent manners.
Although the bands for SP-A (33 kDa) in the kidney extracts were detected by Kankavi [
21], SP-A mRNA was never detected in the renal tissues of mice [
22,
23] and humans. The current study presented the exact expressions of SP-A mRNA and protein in human renal tissues. The different results of the present and previous studies may be attributed to the following. First, the present study performed repetitive experiments and collected more samples than previous studies. Second, compared with previous studies, the present study considered different sites of specimen collection in the renal tissues, where SP-A had a higher level of expression. Third, the nucleotide sequence of SP-A in PUBMED has been revised.
Both SP-A1 and SP-A2 transcripts are expressed in adult human alveolar type II cells [
24]. McCormick et al. [
24] reported that 65% of the SP-A mRNA is encoded by the SP-A2 gene, whereas only 35% is derived from the SP-A1 gene in the lungs. The SP-A1 and SP-A2 genes are differentially expressed in different tissues. Only the SP-A2 gene is predominantly detected in the trachea [
25] and submucosal gland cells in the airway [
20], whereas SP-A1 and SP-A2 transcript expressions are both detected in the small and large intestines of humans [
26]. If the SP-A1 gene is only expressed, then the SP-A cDNA fragment (439 bp) can be digested by Apa I. In this study, the PCR products (439 bp) of the renal tissues and HK-2 cells were digested to 217 and 222 bp bands (bands overlapped at 220 bp). This finding indicated that the SP-A1 gene can be expressed in the renal tissues and HK-2 cells. We also used another primer pair that is common to SP-A1 and SP-A2 (295 bp) to amplify the SP-A cDNA segments of the HK-2 cells and then performed direct sequencing. The sequencing data, which were evaluated by the BLAST tool on PUBMED, correspond to the expected sequences of SP-A1 and SP-A2. The primer pairs specific to SP-A1 or SP-A2 were also used to identify the expressions of the SP-A1 and SP-A2 genes. Considering the result obtained from the Apa I digestion experiment, we conclude that the SP-A1 and SP-A2 genes were expressed in the renal tissues and HK-2 cells in the same way as in the alveolar type II cells. However, the SP-A mRNA level was relatively reduced in the renal tissues and HK-2 cells than in the lungs. We did not determine whether the surface area of the urinary tract is smaller, although the SP-A gene expression in the renal tissue was found to be much lower, which may still be enough to function in local host defence.
In the present study, we have shown that both SP-A1 and SP-A2 mRNA is expressed in renal tissue and the HK-2 cell line. As the SP-A protein can be detected by the polyclonal antibody of SP-A as well in renal tissue and the HK-2 cell line, as shown by western blotting and immunohistochemistry, the polyclonal antibody could potential recognise epitopes in both the SP-A1 and SP-A2 proteins. Therefore, the localisation and synthesis of SP-A occur in the kidneys. Immunostained SP-A is present in the epithelial cells of different tissues, such as in the Eustachian tube [
12] and nasal cavities [
27]. Immunoreactive SP-A is also found in human Eustachian tube lavage [
12] and middle ear fluids [
27]. We frequently detected that the renal tubular epithelial cells contain the SP-A protein, which is in good agreement with the findings of a previous study [
21].Gram-negative bacteria, such as E. coli, are one of the major causes of urinary tract infection. LPS is the major component of
E.
coli. Thus, the severity and time course of kidney inflammation may depend on the amount of LPS. SP-A is the most abundant surfactant protein in the lungs and contributes to lung host defence. A previous study reported that SP-A gene knocked-out mice are susceptible to lung infection caused by several pathogens. In the present study, the levels of SP-A1 and SP-A2 mRNA and protein in the HK-2 cells were significantly increased after LPS treatment. This finding indicated that SP-A may play an anti-inflammatory role in kidney infection.
In summary, the following conclusions are presented. First, human renal tubular epithelial cells can transcribe both SP-A1 and SP-A2 genes. Second, LPS induces SP-A1 and SP-A2 mRNA and protein syntheses in time- and dose-dependent manners. Third, SP-A in the renal tissues may prevent the spread of specific infections from the urinary tract to other body parts. However, the mechanism should be further studied.
Competing interests
The authors declare that they have no competing interests.
Authors’ contributions
JL carried out the cell incubation experiment, SP-A1/SP-A2 detection and drafted the manuscript. FQH carried out the SP-A1/SP-A2 expression induced by LPS. GRW participated in the design of the study. QSZ performed the statistical analysis. GHD conceived of the whole study, participated in its design and coordination. All authors read and approved the final manuscript.