ARTICLE |
Correspondence to: Hiromichi Tsurui, Dept. of Pathology, Juntendo University School of Medicine, 2-1-1 Hongo, Bunkyo-Ku, Tokyo 113-8421, Japan. E-mail: tsurui@med.juntendo.ac.jp
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Summary |
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Seven-color analyses of immunofluorescence-stained tissue samples were accomplished using Fourier spectroscopy-based hyperspectral imaging and singular value decomposition. This system consists of a combination of seven fluorescent dyes, three filtersets, an epifluorescence microscope, a spectral imaging system, a computer for data acquisition, and data analysis software. The spectra of all pixels in a multicolor image were taken simultaneously using a Sagnac type interferometer. The spectra were deconvolved to estimate the contribution of each component dye, and individual dye images were constructed based on the intensities of assigned signals. To obtain mixed spectra, three filter sets, i.e., Bl, Gr, and Rd for Alexa488 and Alexa532, for Alexa546, Alexa568, and Alexa594, and for Cy5 and Cy5.5, respectively, were used for simultaneous excitation of two or three dyes. These fluorophores have considerable spectral overlap which precludes their separation by conventional analysis. We resolved their relative contributions to the fluorescent signal by a method involving linear unmixing based on singular value decomposition of the matrices consisting of dye spectra. Analyses of mouse thymic tissues stained with seven different fluorescent dyes provided clear independent images, and any combination of two or three individual dye images could be used for constructing multicolor images. (J Histochem Cytochem 48:653662, 2000)
Key Words: fluorescence image, multicolor imaging, hyperspectral imaging, Fourier spectroscopy, singular value decomposition, linear unmixing
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Introduction |
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Over the past two decades, much of the progress in biology and pathology has resulted from the identification and characterization of new functional molecules within cells. With suspension cells, flow cytometry has provided a means for the simultaneous identification of as many as 10 different proteins within single cells (
Functional maturation and effector functions of immune cells occur through interactions of different cell populations in particular microenvironments. Therefore, identifications of a variety of functionally distinct cell types and their localization in tissues are essential for estimating events occurring in vivo. At present, filter-based isolation of fluorescence signals is the prevalent system for multicolor analysis of different cell types in tissues. However, if emission spectra of different dyes are overlapping, individual filter-passed signals and standard detectors will yield mixed signals. Therefore, the fluorochromes used in this type of analysis are chosen for their lack of overlap with the other fluorochromes used in the analysis. Because the numbers of dyes with adequately wide and intense non-overlapping emission spectra are limited, the complexity of multicolor analysis of tissues has been restricted.
Recent progress in instrumentation, fluorescent dyes, and computer software for numerical analysis has allowed the development of new approaches for multicolor analysis in which the spectrum of a dye mixture can be expressed as a linear combination of the component dye spectra. The signal intensity of each dye can therefore be precisely determined from a single composite spectrum. An interferometric imaging spectrometer (SD-200) (Applied Spectral Imaging; Migdal Haemek, Israel) has recently been introduced in laboratory use (
Combining an efficient imaging spectrometer, appropriate dyes, suitably designed filter sets, and a signal isolation algorithm, we have developed a seven-color fluorescence imaging system for analysis of tissue specimens.
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Materials and Methods |
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Reagents
Succinimidyl ester dyes Alexa488, Alexa532, Alexa546, Alexa568, and Alexa594 and succinimidyl ester dyes Cy5 and Cy5.5 were purchased from Molecular Probes (Eugene, OR) and from Amersham Pharmacia Biotech (Uppsala, Sweden), respectively. Monoclonal antibodies (MAbs) to CD4 (RM4-5), CD8 (53-6.7), CD11c (HL3), CD18 (M18/2), CD44 (IM7), CD45R (RA3-6B2), T-cell receptor ß-chain (ßTCR, H57-597), and I-Ad /I-Ed (2G9) were purchased from BD PharMingen (Franklin Lakes, NJ). NHS-biotin and streptavidin were from Vector Laboratories (Burlingame, CA), NHS-digoxigenin and goat anti-digoxigenin antibodies from Roche Diagnostics (Mannheim, Germany). For staining of single-cell suspensions, MAb 6B2 was labeled with all the dyes except Cy5.5. Cy5.5 was indirectly stained using biotinylated antibodies and Cy5.5-labeled streptavidin. For tissue staining, MAbs against CD4, CD8, CD11c, I-Ad /I-Ed, and ßTCR were labeled with Cy5, Alexa488, Alexa546, Alexa568, and Alexa594, respectively. The MAbs anti-CD18 and anti-CD44 were modified with NHS-digoxigenin and NHS-biotin, respectively. Streptavidin and anti-digoxigenin were labeled with Cy5.5 and Alexa532, respectively. All conjugations were performed in our laboratory according to the manufacturers' instructions.
Filter Design
Three filter sets, designated Bl, Gr, and Rd were designed. Spectral features of the dyes are shown in Table 1, and the construction of the filter sets is shown in Table 2. Bl was used for Alexa488 and Alexa532, Gr was for Alexa546, Alexa568, and Alexa594, and Rd was for Cy5 and Cy5.5. All the filters were purchased from Omega Optical (Brattleboro, VT) and assembled in filter cubes from Olympus (Tokyo, Japan).
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Instrumentation
Imaging spectrometer SD-200 was purchased from Applied Spectral Imaging. Details of the structure and the principle for data acquisition have been reported elsewhere (
Signal Isolation
The spectrum of each pixel was expressed as a linear combination of the spectra of component dyes, using the formula shown in Fig 1A. To obtain the abundance vector, the observed spectra were multiplied on the left by a "generalized inverse" of the spectral matrix according to
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Sample Preparation
Mice were treated according to the guidelines of Juntendo University Animal facility. Spleen cell suspensions in isotonic PBS, pH 7.4, were prepared from 2-month-old Balb/c mice by gently dispersing cells from tissues using a glass tissue grinder. Cells were stained single-colored, double-colored, and triple-colored with MAb 6B2 conjugated with different fluorochromes. Ten µl of the suspension of stained cell was dropped on a slide glass, sealed with a coverslip, and submitted to analysis. For tissue multicolor immunofluorescence analyses, thymic tissues from 2-month-old New Zealand Black mice were embedded in OCT compound (Miles Scientific; Naperville, IL) and rapidly frozen in liquid nitrogen. Cryostat sections 2 µm thick were fixed in acetone for 10 min and air-dried for 3 min. After immersing in PBS for 5 min, the tissue sections were treated with appropriate concentrations of all antibodies simultaneously, left at room temperature (RT) for 30 min with occasional agitation, washed with PBS, stained with second reagents for 30 min at RT, washed three times with PBS, and sealed with Gel/Mount (Biomeda; Foster City, CA) and a coverslip. The staining reagents contained 0.2% of bovine serum albumin (BSA), 0.05% of Tween-20, and 0.05% of sodium azide. No anti-fade reagent was used.
Data Acquisition and Analysis
Spectral images of blank glass were used as background images. Background images were subtracted from those of all spectral images of samples before analysis. For the construction of spectral libraries, the spectrum of each dye was obtained by averaging signals from the six brightest points in a spectral image of single-stained cells. Linear unmixing based on SVD was performed using these spectral libraries as references. For seven-color imaging, spectral images using Bl, Gr, and Rd filter sets were taken sequentially for one field. After analysis, three of seven decomposed images were used to construct a multicolor image.
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Results |
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In the system we designed, appropriate filter sets are essential. They are required to excite dyes as efficiently as possible, to remove scattered excitation light completely, and to acquire emission spectra as broad as possible. On the basis of spectral features and absorption and emission spectra, shown in Table 1 and Fig 2A2F, respectively, seven dyes were selected and separated into Bl, Gr, and Rd dye groups. Even though absorption spectra and emission spectra of dyes in each group, particularly in group Bl, were very close (Fig 2A2F), the exciter, dichroic mirror, and the emitter filters were required to pass rather broad wavelength regions to realize efficient excitation and light collection. Although the use of these filters caused attenuation of the signal intensity in the short-wavelength portion of each emission region, we could minimize this problem by selection and combination of filters that balance efficient excitation and signal acquisition for each dye group. The spectra of excitation filters used are shown in Fig 2A2C and those of emission filters are shown in Fig 2D2F. Exciters, dichroic mirrors, and emitters with steep edges, regions of transmissions closely spaced for simultaneous excitation and acquisition of wide spectra, were selected. (Spectra of dichroic mirrors are not shown.) The spectrum of each dye was obtained by averaging the six brightest points in the image of single-color stained cells (Fig 2G2I , dotted lines).
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As can be seen in Fig 2A, Fig 2B, Fig 2D, and Fig 2E, Alexa532 is efficiently excited with filter set Gr and its longer-wavelength portion of emission passes through this filter-set. Therefore, simultaneous staining of specimens with dyes of both Bl and Gr gave a false- positive estimate for Alexa546. A similar but lesser problem occurred with Alexa594 showing up in the Rd measurements (Fig 2B, Fig 2C, Fig 2E, and Fig 2F). We avoided this problem by adding adequate dummy exposure after image acquisition using Bl and Gr; hence, no false-positive signal from shorter wavelength dye groups affected the following measurements.
Spectra thus obtained were fairly close to those previously published ( http://www.probes.com), but there were several differences between the observed and the published spectra. Emission spectra of Alexa488, Alexa546, and Cy5 were apparently shifted to longer wavelengths (to the right) than were found in the published data. This appeared to be mainly due to the blocking of signals in shorter-wavelength regions by the emitter filter (Fig 2D2I). The spectrum of Cy5.5 appeared to be shifted to shorter wavelengths (to the left). This was due to the decreasing quantum yields of the CCD at long wavelengths. All the spectra observed were wider than those seen in the published data. This can be ascribed to the heterogeneity of dye microenvironments. Because of these three effects, spectra of dyes in the same group were less well separated than expected (Fig 2G2I). However, they were found to be useful for practical analyses. The spectra thus obtained from images served as spectral libraries for linear unmixing based on SVD.
To confirm the linearity of fluorescence image composition and the validity of SVD for signal isolation, we first examined spectral images of spleen cell suspensions from untreated Balb/c mice 2 months of age, single, double, or triple stained with B-lymphocyte-specific MAb 6B2 (anti-CD45R) conjugated with different dyes in the same group. Spectral images of stained cell suspensions were corrected by subtracting background images of a blank slide glass with coverslip, and were subjected to linear unmixing based on SVD.
Fig 3 shows representative results of single-color stained cells, indicating that each dye signal was clearly isolated. The signal image of a cell stained with a dye was seen only on the "axis" of that dye. This was confirmed by experiments in which aliquots of spleen cell suspension were separately stained with different dyes in the same group (not shown).
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Strict signal isolation was also observed with cells either double or triple stained with different dyes in the same group. The images of cells were projected onto "axes" of dye spectra used for staining ( Fig 4), thus providing evidence that signals from the same point can be isolated independently and that dyes in a particular location do not affect each other.
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On the basis of these findings, we tested the method in seven-color fluorescence imaging of thymic tissue samples obtained from a 2-month-old New Zealand Black mouse. Frozen sections of the thymus were stained simultaneously with seven different reagents, each conjugated with a different dye or hapten. Reagents used were anti-CD8 (Alexa488), anti-CD18 (Alexa532), anti-CD11c (Alexa546), anti-I-Ad/I-Ed (Alexa568), anti-ßTCR (Alexa594), anti-CD4 (Cy5), and anti-CD44 (Cy5.5).
Precursors of T-cells migrate into the thymus, differentiate, and mature there before moving into the systemic circulation. CD4- CD8- cells in early development can be divided into four stages according to the expression of CD25 and CD44; CD44+ CD25-, CD44+ CD25+, CD44 - CD25+, and CD44- CD25 - (-chains are expressed, and cells expressing complete TCR undergo apoptosis or maturation to CD4 + CD8- cells and CD4- CD8 + cells according to the interaction between Class I and Class II molecules expressed on thymic epithelial cells (
D-subunit, resulting in the formation of LFA-1, Mac-1, p150, 95, and
Dß2, respectively. CD11c is expressed on macrophages, dendritic cells, and NK cells.
Signals of Alexa532 and Cy5.5 were amplified by the digoxigeninanti-digoxigenin system and the biotinavidin system, respectively. All other dyes were conjugated directly to the antibodies. After staining, spectral images for Bl, Gr, and Rd group dyes were taken sequentially in the order listed, using corresponding filter sets. In these measurements, dummy exposures were added to remove the false-positive signals from the shorter-wavelength dye groups. Spectral images were analyzed by linear unmixing based on SVD, referring to the spectral libraries previously constructed. We confirmed beforehand that Gel/Mount had no effect on the dye spectra (not shown).
Fig 5 shows that all the signals from these dyes were isolated independently. Medulla, the spreading lower left portion in the image, is surrounded by cortex. ßTCRs are expressed more strongly in the medulla than in the cortex, whereas CD4+ cells and CD8+ cells are sparse in the medulla. I-Ad /I-Ed is expressed on epithelial cells in both cortex and medulla, in a different distribution pattern. CD44+ cells are distributed mainly in the medulla region. CD18 is mainly expressed on thymocytes both in the cortex and, much more strongly, in the medulla. CD11c is expressed on some populations of CD18+ cells.
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Because independent colors included in a color image are limited to three, three different images in Fig 5 were combined to construct multicolor images (Fig 6E ). Fig 6A6C show three-color images of thymus tissue representing different combinations of the seven reagents. In Fig 6A, CD4 (Cy5), CD8 (Alexa488), and ßTCR (Alexa594) molecules are assigned blue, red, and green, respectively. The cortex is densely occupied with CD4+ CD8+ cells (either white or violet due to a relatively low expression of ßTCR), whereas the medulla shows sparse distribution of the single positive cells (yellow for CD4- CD8+ and cyan for CD4+ CD8-). The distribution of these cells clearly demonstrates the maturation of thymocytes from CD4+ CD8+ cells in the cortex to CD4 + CD8- or CD4- CD8+ cells in the medulla. In Fig 6B, ßTCR (Alexa594), I-Ad/I-Ed (Alexa 568), and CD44 (Cy5.5) are assigned to green, red, and blue, respectively. I-Ad /I-Ed is strongly expressed in the cortex, where expression of ßTCR is relatively low. Some CD44+ cells do not overlap ßTCR-expressing cells, suggesting them to be macrophages. As shown in Fig 6C, in which CD18 (Alexa532), ßTCR (Alexa594), and CD11c (Alexa546) molecules are assigned to red, green, and blue in the image, respectively, the medulla displays preferential accumulation of CD18 high ßTCR+ thymocytes (yellow), and the cortex is mainly composed of CD18 low ßTCR+ thymocytes. CD11c is expressed on some portions of CD18+ cells (violet).
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Discussion |
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In the present studies, using properly selected dyes, suitably designed filter sets, and a sophisticated mathematical analysis in combination with a recently developed imaging spectrometer, we designed a seven-color fluorescence imaging method for immunostained tissue samples. For dyes, efforts were made to select those with properties of strong signal intensity, low nonspecific binding to tissues, and flexibility of protein modification. We used Alexa488, 532, 546, 568, and 594 for emission at wavelengths from 500 to 650 nm. Among a variety of dyes with emission spectra similar to Alexa series, fluorescein and FluorX (Amersham Pharmacia Biotech) had similar spectral features to Alexa488. However, both showed weaker signals and were less photostable than Alexa488. Addition of P-phenylenediamine reduced the photobleaching of fluorescein. However, it considerably broadened the emission spectrum (not shown). Phycoerythrin had an acceptable emission spectrum and a strong signal, but it bleached rapidly. Cy series of dyes Cy2, Cy3, and Cy3.5 (Amersham Pharmacia Biotech) have appropriate emission spectra. However, rates of photobleaching were all far higher than those found in Alexa series dyes (not shown). Texas Red rendered conjugates sticky, causing all the labeled antibodies to agglutinate. In the Alexa series, although Alexa546 was difficult to excite simultaneously with Alexa488, it could be excited efficiently with Alexa594 (Fig 2A and Fig 2B). For dyes to be excited at longer wavelengths, we used Cy5 and Cy5.5. These two dyes showed sufficiently separate spectra, generated fairly strong signals, and gave clear images when measured with a Photometrics PXL1400 camera (not shown). However, because the cooled CCD camera attached to SD-200 had a low sensitivity at long wavelengths, we amplified the signal of Cy5.5 using the biotin-streptavidin system. Cy7 has a spectrum well separated from those of Cy5 and Cy5.5 (maximal absorption is at 743 nm and maximal emission is at 767 nm). However, it was not excited efficiently with the high-pressure mercury lamp, and the sensitivity of the CCD camera at this wavelength was very low.
Many factors were found to affect the shape of observed spectra, i.e. emission filters, the dependence of the CCD camera quantum yield on wavelength, and the microenvironment of the dyes. Because shorter-wavelength regions of the emission spectra of Alexa488, Alexa546, and Cy5 were blocked by the emission filters (Fig 2D2F), an apparent shift of the emission peaks to longer wavelength occurred. The spectrum of Alexa546 obtained using a filter set with lower pass region is quite similar to the published spectrum (not shown). Most of the observed distortion of these dye spectra can be ascribed to this effect. Indeed, the spectra of Alexa568, Alexa594, and Cy5.5 did not show peak shifts to the longer wavelength. Rather, the spectrum of Cy5.5 was shifted to a shorter wavelength. Because of the decreasing quantum yield of CCD camera with increasing wavelength (from 26% at 650 nm to 14% at 750 nm), the measured spectral peak was shifted to a shorter wavelength. Microenvironments of dyes in tissue samples vary among the dye molecules, resulting in subtle difference in emission spectra to broadening of the averaged spectra. We examined images of mixtures of cell suspensions single-color stained with Alexa488 and Alexa532 using very sensitive similarity mapping method. Spectra from cells stained with each dye were divided into four or five classes, and no spectrum was observed in both the regions (not shown). Small variance of spectra from images was observed by another method (
In fluorescence images, the principle of superposition is generally valid. In other words, a fluorescence image behaves like a vector space or, more precisely, a convex body (
A karyotyping method based on spectral imaging and combinatorial chromosome staining (spectral karyotyping, SKY) distinguishes 24 human chromosomes, including two sex chromosomes. The principle of this method is to measure spectral angles between the spectrum of the chromosome and those of endmembers of the library and to assign the chromosome's spectrum to the nearest endmember (
The similarity mapping method measures the distance between the spectra of pixels and classifies them by grouping the nearest ones (
Photobleaching inevitably occurs during the data collection, making it difficult to obtain high-quality spectra from fluorescence images. To minimize this effect, an instrument with high throughput and efficient signal collection is required. In this regard, monochrometers and bandpass filters are not optimal for fluorescence spectral imaging because only limited portions of emission signals are passed, leading to low quality of acquired spectra and long times for data collection. In this context, the interferometric method works well because of its high throughput and rapid data collection.
As is demonstrated by commonly performed karyotyping, spectral imaging based on the interferometric method provides fairly high resolution at strong magnification. We obtained complete isolation of dye signals used in this study with a x40 objective lens (not shown). These facts suggest the probability that this method can be applied to cytological investigations.
The multicolor fluorescence imaging method we designed in the present study may be useful for elucidating complex structures consist of several kinds of components or cells that are not distinguishable simultaneously by other means. Furthermore, co-measurement of several factors in an image is available only with this method. Hence, it may be useful for investigating the interactions among several molecules in a cell and, with the help of FACS, for evaluating the role of particular cells in tissue characterized by several markers.
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Acknowledgments |
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We wish to thank to Dr Michael T. Anderson for critical reading of the manuscript and correction of the English. We also thank Sumitomo Electric Industries, Ltd., for the loan of a laboratory room.
Received for publication January 14, 2000; accepted January 19, 2000.
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