Comparison of ophthalmic sponges and extraction buffers for quantifying cytokine profiles in tears using Luminex technology

Purpose Evaluating cytokine profiles in tears could shed light on the pathogenesis of various ocular surface diseases. When collecting tears with the methods currently available, it is often not possible to avoid the tear reflex, which may give a different cytokine profile compared to basal tears. More importantly, tear collection with glass capillaries, the most widely used method for taking samples and the best method for avoiding tear reflex, is impractical for remote area field studies because it is tedious and time-consuming for health workers, who cannot collect tears from a large number of patients with this method in one day. Furthermore, this method is uncomfortable for anxious patients and children. Thus, tears are frequently collected using ophthalmic sponges. These sponges have the advantage that they are well tolerated by the patient, especially children, and enable standardization of the tear collection volume. The aim of this study was to compare various ophthalmic sponges and extraction buffers to optimize the tear collection method for field studies for subsequent quantification of cytokines in tears using the Luminex technology. Methods Three ophthalmic sponges, Merocel, Pro-ophta, and Weck-Cel, were tested. Sponges were presoaked with 25 cytokines/chemokines of known concentrations and eluted with seven different extraction buffers (EX1–EX7). To assess possible interference in the assay from the sponges, two standard curves were prepared in parallel: 1) cytokines of known concentrations with the extraction buffers and 2) cytokines of known concentrations loaded onto the sponges with the extraction buffers. Subsequently, a clinical assessment of the chosen sponge-buffer combination was performed with tears collected from four healthy subjects using 1) aspiration and 2) sponges. To quantify cytokine/chemokine recovery and the concentration in the tears, a 25-plex Cytokine Panel and the Luminex xMap were used. This platform enables simultaneous measurement of proinflammatory cytokines, Th1/Th2 distinguishing cytokines, nonspecific acting cytokines, and chemokines. Results We demonstrated the following: (i) 25 cytokines/chemokines expressed highly variable interactions with buffers and matrices. Several buffers enabled recovery of similar cytokine values (regulated and normal T cell expressed and secreted [RANTES], interleukin [IL]-13, IL-6, IL-8, IL-2R, and granulocyte-macrophage colony-stimulating factor [GM-CSF]); others were highly variable (monocyte chemotactic protein-1 [MCP-1], monokine induced by interferon-gamma [MIG], IL-1β, IL-4, IL-7, and eotaxin). (ii) Various extraction buffers displayed significantly different recovery rates on the same sponge for the same cytokine/chemokine. (iii) The highest recovery rates were obtained with the Merocel ophthalmic sponge except for tumor necrosis factor-α: the Weck-Cel ophthalmic sponge showed the best results, either with cytokine standards loaded onto sponges or with tears collected from the inner canthus of the eye, using the sponge. (iv) IL-5, IL-10, and interferon-α were not detected in any tear sample from four normal human subjects. Twenty-two cytokines/chemokines that we detected were extracted from the Merocel sponge to a satisfactory recovery percentage. The recovery of IL-7 was significantly lower in the extracted Merocel sponge compared to the diluted tear samples. The cytokine/chemokine extraction from tears showed the same pattern of extraction that we observed for extracting the standards. Conclusions Simultaneous measurement of various cytokines using ophthalmic sponges yielded diverse results for various cytokines as the level of extraction differs noticeably for certain cytokines. A second set of controls (standard curves “with sponges”) should be used to delineate the extent of extraction for each cytokine to be analyzed. Many cytokines/chemokines were detected in tear samples collected with the Merocel sponge, including many that have been implicated in ocular surface disease. Luminex detection of cytokine/chemokine profiles of tears collected with Merocel sponges and extracted with buffer EX1 may be useful in clinical studies, for example, to assess cytokine profiles evaluation in ocular surface diseases.

[1]  R. Casson,et al.  Interleukin-6 is an efficacious marker of axonal transport disruption during experimental glaucoma and stimulates neuritogenesis in cultured retinal ganglion cells , 2012, Neurobiology of Disease.

[2]  S. Bonini,et al.  Molecular and cellular biomarkers in dry eye disease and ocular allergy , 2012, Current opinion in allergy and clinical immunology.

[3]  C. Joo,et al.  Correlations between tear cytokines, chemokines, and soluble receptors and clinical severity of dry eye disease. , 2012, Investigative ophthalmology & visual science.

[4]  R. Adelman,et al.  Effects of proinflammatory cytokines on the claudin-19 rich tight junctions of human retinal pigment epithelium. , 2012, Investigative ophthalmology & visual science.

[5]  K. Ward,et al.  A method to extract cytokines and matrix metalloproteinases from Schirmer strips and analyze using Luminex , 2011, Molecular vision.

[6]  Y. Chun,et al.  Tear cytokines and chemokines in patients with Demodex blepharitis. , 2011, Cytokine.

[7]  S. Whitcup,et al.  Cytokine and chemokine levels in tears from healthy subjects , 2010, Acta ophthalmologica.

[8]  M. Senchyna,et al.  Tear lipocalin and lysozyme concentrations in postmenopausal women , 2010, Ophthalmic & physiological optics : the journal of the British College of Ophthalmic Opticians.

[9]  M. Esmaeelpour,et al.  Tear sample collection using cellulose acetate absorbent filters , 2008, Ophthalmic & physiological optics : the journal of the British College of Ophthalmic Opticians.

[10]  Elena Vecino,et al.  Inflammatory Markers in the Tears of Patients with Ocular Surface Disease , 2008, Ophthalmic Research.

[11]  Gerhard Walzl,et al.  An Evaluation of Commercial Fluorescent Bead-Based Luminex Cytokine Assays , 2008, PloS one.

[12]  R. López-Solís,et al.  Use of Polyurethane Minisponges to Collect Human Tear Fluid , 2006, Cornea.

[13]  W. Hop,et al.  Multiplex Bead Array Assay for Detection of 25 Soluble Cytokines in Blister Fluid of Patients with Complex Regional Pain Syndrome Type 1 , 2006, Mediators of inflammation.

[14]  Prof. Otto Schirmer Studien zur Physiologie und Pathologie der Tränenabsonderung und Tränenabfuhr , 1903, Albrecht von Graefes Archiv für Ophthalmologie.

[15]  P. Castle,et al.  Comparison of Ophthalmic Sponges for Measurements of Immune Markers from Cervical Secretions , 2004, Clinical Diagnostic Laboratory Immunology.

[16]  Savitri Sharma,et al.  Is the cystatin-like domain of TSL functionally active in external ocular infections and during the normal diurnal cycle? , 2004, Experimental eye research.

[17]  E. Partridge,et al.  Rectal Immunization for Induction of Specific Antibody in the Genital Tract of Women , 1997, Journal of Clinical Immunology.

[18]  D. Tang-Liu,et al.  Comparison of tear sampling techniques for pharmacokinetics analysis: ofloxacin concentrations in rabbit tears after sampling with schirmer tear strips, capillary tubes, or surgical sponges. , 2000, Journal of ocular pharmacology and therapeutics : the official journal of the Association for Ocular Pharmacology and Therapeutics.

[19]  N. Occleston,et al.  Sponge delivery variables and tissue levels of 5-fluorouracil , 2000, The British journal of ophthalmology.

[20]  L. Kelly,et al.  Optimization of the Weck-Cel Collection Method for Quantitation of Cytokines in Mucosal Secretions , 2000, Clinical Diagnostic Laboratory Immunology.

[21]  C. Svanborg,et al.  Cytokine responses during mucosal infections: role in disease pathogenesis and host defence. , 1999, Current opinion in microbiology.

[22]  S. Shivaji,et al.  HPLC analysis of closed, open, and reflex eye tear proteins. , 1998, Indian journal of ophthalmology.

[23]  T. Flanigan,et al.  Comparison of the oral, rectal, and vaginal immunization routes for induction of antibodies in rectal and genital tract secretions of women , 1997, Infection and immunity.

[24]  Mark J. Mannis,et al.  Duane's Ophthalmology , 1993 .

[25]  A. Wlodawer,et al.  Hematopoietic cytokines: Similarities and differences in the structures, with implications for receptor binding , 1993, Protein science : a publication of the Protein Society.

[26]  Martin W. Bloem,et al.  Recovery of protein from tear fluid stored in cellulose sponges. , 1987, Current eye research.

[27]  M. Becker The Lacrimal Drainage System , 1986 .