Quantitating fluorescence intensity from fluorophore: the definition of MESF assignment.The quantitation of fluorescence fluorescence (fl  rĕs`əns), luminescence in which light of a visible color is emitted from a substance under stimulation or excitation by light or other forms of electromagnetic radiance may at first suggest the need to obtain the number of fluorophore that are responsible for the measured fluorescence radiance. This goal is beset by many difficulties since the fluorescence radiance depends on three parameters 1) the probability of absorbing a photon (molar molar /mo·lar/ (mo´lar)1. pertaining to a mole of a substance. 2. a measure of the concentration of a solute, expressed as the number of moles of solute per liter of solution. Symbol M, , or mol/L. extinction), 2) the number of fluorophores, and 3) the probability of radiative decay of the excited state (quantum yield The quantum yield of a radiation-induced process is the number of times that a defined event occurs per photon absorbed by the system. Thus, the quantum yield is a measure of the efficiency with which absorbed light produces some effect. ). If we use the same fluorophore in the reference solution and the analyte then, to a good approximation, the molar extinction drops out from the comparison of fluorescence radiance and we are left with the comparison of fluorescence yield which is defined as the product of fluorophore concentration and the molecular quantum yield. The equality of fluorescence yields from two solutions leads to the notion of equivalent number of fluorophores in the two solutions that is the basis for assignment of MESF MESF Mobile Electronics and Security Federation (UK trade association) MESF Maritime Expeditionary Security Force MESF Minimum Engineered Safety Feature (Molecules of Equivalent Soluble Fluorophore) values. We discuss how MESF val ues are assigned to labeled microbeads and by extension to labeled antibodies, and how these assignments can lead to the estimate of the number of bound antibodies in flow cytometer measurements. Key words: flow cytometer; fluorescein fluorescein /flu·o·res·ce·in/ (fldbobr-res´en) a fluorescing dye; its sodium salt is used as a tracer in retinal angiography and as a diagnostic aid for revealing corneal trauma and fitting contact lenses. ; fluorescence; MESF; microbeads; quantitation; SRM (1) (Storage Resource Management) The management of the storage resources in an organization in order to avoid duplication of files and to determine space utilization across all servers. 1932. 1. Introduction The number of fluorescence based assays has grown rapidly in the last 20 years, especially in the fields of biological research and clinical diagnosis (1). The growth has been driven by the rapid developments in fluorophore conjugation conjugation, in genetics conjugation, in genetics: see recombination. conjugation, in grammar conjugation: see inflection. chemistry (2) and by the high inherent sensitivity of fluorescence measurement (down to a few hundred fluorophores or less) (3, 4). With the proper use of standards the fluorescence intensity can be quantitated yielding further utility to fluorescence based assays (5-7). Soluble analytes can be quantitated using reference materials dissolved in the same media as the analyte. In such cases the molar extinction and quantum yield of the fluorophore is the same for the analyte and the reference material and the fluorescence radiance from both is proportional to the relative number of fluorophores. In the case where one set of fluorophores is in solution and the other set of fluorophores is immobilized on a microbead, the quantum yields may be different for the two fluorophores and the equality of fluorescence radiance does not imply equal numbers of fluorophores. In what follows we discuss the notion of MESF (Molecules of Equivalent Soluble Fluorophore) as a method for quantitating fluorescence radiance in the case where quantum yields differ between the analyte and the reference solution. The discussion below is based on the concept of fluorescence yield which is defined as the product of the fluorophore concentration and the quantum yield of the fluorophore. The quantum yield is defined as the ratio of the number of photons emitted by a fluorophore to the number of photons absorbed by the fluorophore. In the same spirit the fluorescence yield of a solution is a measure of the number of photons emitted per unit volume if every fluorophore absorbs a photon. For fixed solution conditions the fluorescence yield is a well-defined property of the solution. Just as it is valid to compare the quantum yield of two fluorophores, it is also valid to compare the fluorescence yield of any two solutions. Experience has shown that the quantum yield and hence the fluorescence yield is a highly variable property of the fluorophore's microenvironment microenvironment /mi·cro·en·vi·ron·ment/ (-en-vi´ron-ment) the environment at the microscopic or cellular level. . For example, due to the existence of multiple forms of fluorescein, the apparent quantum yield of fluorescein changes from 0.93 to 0.37 when the buffer pH goes f rom 9 to 5 (8,9). Similarly the fluorescence yield of the solution would change upon a change in pH. Conjugating a fluorophore to a protein (10) or DNA DNA: see nucleic acid. DNA or deoxyribonucleic acid One of two types of nucleic acid (the other is RNA); a complex organic compound found in all living cells and many viruses. It is the chemical substance of genes. (11) usually changes its quantum yield. Hence it was realized early that trying to quantitate quan·ti·tate tr.v. quan·ti·tat·ed, quan·ti·tat·ing, quan·ti·tates To determine or measure the quantity of. [Back-formation from quantitative (analysis). fluorescence intensity in terms of an actual number of fluorophores is a difficult task. The notion of fluorescence yield allows solutions to be compared in a meaningful way and is the basis for the notion of MESF which has been used as a practical method for quantitating fluorescence radiance. In what follows we will discuss the concept of fluorescence yield, how it leads to MESF, the actual assignment of the MESF value, and finally some cautionary remarks on the variation expected in practical assignment of the MESF values. 2. Comparison of Fluorescence Yields The fluorescence yields will be compared relative to a standard reference solution of a fluorophore such as fluorescein. The reference solution will serve as a "meter stick" to which all other fluorescence yields will be compared. The fluorescence yield will be obtained from a measurement of fluorescence radiance. In the following we use the term "fluorescence intensity" and fluorescence signal interchangeably, both denote the output of a detection system that measures the radiation from a fluorescing sample. The measurements will be carried out using a conventional fluorimeter fluorimeter /flu·o·rim·e·ter/ (fldbobr-rim´e-ter) fluorometer. fluorimeter see fluorometer. consisting of a monochromator A monochromator is an optical device that transmits a mechanically selectable narrow band of wavelengths of light or other radiation chosen from a wider range of wavelengths available at the input. with a CCD CCD in full charge-coupled device Semiconductor device in which the individual semiconductor components are connected so that the electrical charge at the output of one device provides the input to the next device. detector at the exit slit, and a source consisting of a cuvette cuvette /cu·vette/ (ku-vet´) [Fr.] a glass container generally having well-defined characteristics (dimensions, optical properties), to contain solutions or suspensions for study. cu·vette n. with a illumination region parallel to the entrance slit of the monochromator. A schematic of the apparatus is shown in Fig. 1. The measurement of the fluorescence radiance will be performed by combining the fluorescence signal from the fluorescing source at wavelength [[lambda].sub.0] [S.sub.f]([[lambda].sub.0]), and signal from a radiance standard, S'([[lambda].sub.0]). The two measured signals will be combined as shown in Eq. (1) where L'([[lambda].sub.0]) is the known radiance of the standard source and [L.sub.f]([[lambda].sub.0]) is the unknown radiance of the fluorescing sample. This combination of the measured signals provides a correction for instrument spectral response The variable output of a light-sensitive device that is based on the color of the light it perceives. . The measured fluorescence spectral radiance is given in terms of measured signals by (Eq. (A13) in the Appendix) [L.sub.f][[lambda].sub.0] = [S.sub.f] ([[lambda].sub.0])/ S'([[lambda].sub.0]) L'([[lambda].sub.0]) (1) As shown in the appendix [Eq. (A10)], the spectral radiance [L.sub.f]([[lambda].sub.0]) can also be given in terms of the properties of solution and fluorophore by [L.sub.f]([[lambda].sub.0]) = [I.sub.0]N[OMEGA][epsilon]([[lambda].sub.x])[phi]s([[lambda].sub.0], [[lambda].sub.x]) (2) where [I.sub.0] is the incident power (W), N is the concentration of fluorophores (1/[m.sup.3]), [OMEGA] (1/im sr) is a factor depending on the geometry of the source and the detector, [epsilon][[lambda].sub.x] is the absorptivity ([m.sup.2]), [phi] is the quantum yield, s ([[lambda].sub.0],[[lambda].sub.x] is the relative spectral emission function (1/nm). The relative emission function, s ([[lambda].sub.0], [[lambda].sub.x]) will be normalized so that the integral over all wavelengths is 1. In many cases the emission spectrum emission spectrum: see spectrum. is independent of the excitation wavelength The excitation wavelength describes the light shone on a sample to transfer energy to ("to excite") a light-reactive chemical group in any compound. Its unit is usually given in nanometers (nm). and can be written as a product of a quantum yield and a normalized relative emission function [see Appendix Eq. (A14)]. Physically, when a molecule is excited, some of the energy goes into changing the state of the electron, and the remainder goes into nuclear vibrations. The nuclear vibrations usually dissipate dis·si·pate v. dis·si·pat·ed, dis·si·pat·ing, dis·si·pates v.tr. 1. To drive away; disperse. 2. their excess energy to the surroundings and reach the lowest vibrational state in less than a ps. Thus the emission always occurs from the same equilibrated excited state even if the initial excited state at the instant of photon absorption was different. Molecules in the equilibrated excited states have many relaxation pathways and changes in the relative importance of these pathways may perturb the emission spectrum. We will assume that the emission spectrum is independent of the other non radiative relaxation pathways. The quantum yield is a measure of the relative probability that the excitation excitation Addition of a discrete amount of energy to a system that changes it usually from a state of lowest energy (ground state) to one of higher energy (excited state). For example, in a hydrogen atom, an excitation energy of 10. will relax via a radiative decay (fluorescence) versus the non radiative pathways. In what follows we will compare the fluorescence radiance, [L.sub.f]([[lambda].sub.0]) of two sources that may have different excitation probabilities, different relative emission functions s([lambda]), and different quantum yields, [phi]. The total fluorescence radiance is obtained by summing over all wavelengths resulting in an expression [L.sub.f] = [integral] [S.sub.f]([[lambda].sub.0]/S'([[lambda].sub.0]) L'([[lambda].sub.0])d[[lambda].sub.0] = [OMEGA]N[phi][epsilon]([[lambda].sub.x])[I.sub.0]. (3) In writing Eq. (3), we have used the fact that the sum of s([[lambda].sub.0],[[lambda].sub.x]) over all values of [[lambda].sub.0], gives 1 according to according to prep. 1. As stated or indicated by; on the authority of: according to historians. 2. In keeping with: according to instructions. 3. the definition of s([[lambda].sub.0],[[lambda].sub.x]) in the Appendix. Suppose that we are free to adjust the concentration of fluorophore in one of the solutions and we adjust the concentration so that the two fluorescing sources give the same total fluorescence radiance. Then according to Eq. (3) we can write [L.sub.s1] = [L.sub.s2] [I.sub.0][N.sub.s1][OMEGA][[epsilon].sub.s1]([[lambda].sub.x])[[phi]. sub.s1] = [I.sub.0][N.sub.s2][OMEGA][[epsilon].sub.s2]([[lambda].sub.x])[[phi]. sub.s2] (4) where [L.sub.s1] and [L.sub.s2] are the total fluorescence radiance [Eq. (3)] measured for two fluorophore solutions or suspensions named s1 and s2, respectively. We say that the response of [N.sub.s1] molecules of fluorophore s1 per [m.sup.3] is equivalent to the response of [N.sub.s2] molecules of fluorophore s2 per [m.sup.3]. Assuming that the geometric factor, [OMEGA], and the illumination, [I.sub.0], are the same for both the solution measurements, the equality of total fluorescence radiance implies the following relation [N.sub.s1][[epsilon].sub.s1]([[lambda].sub.x])[[phi].sub.s1] = [N.sub.s2][[epsilon].sub.s2]([[lambda].sub.x]([[phi].sub.s2]. (4a) Equation (4a) shows the well known fact that the fluorescence radiance is determined by the product of three independent variables: the number of fluorophores, the probability of absorbing a photon, and the probability of emitting a photon. Thus if the above measurement is repeated with a different illumination wavelength, the fluorescence radiances will not be equal since the molar absorptivity The molar extinction coefficient, also known as molar absorptivity, is a measure of how strongly a chemical species at a given wavelength absorbs light at that wavelength. will be different. Figure 2 shows the wavelength dependence of the relative absorption of fluorescein in a pH 9 solution. The absorption is a strong function of wavelength and thus the resulting integrated fluorescence radiance will depend on the wavelength of illumination. In order to eliminate the dependence on excitation wavelength, the fluorescence radiance measurement needs to be normalized by molecular absorptivity at the illumination wavelength. Such a normalization In relational database management, a process that breaks down data into record groups for efficient processing. There are six stages. By the third stage (third normal form), data are identified only by the key field in their record. leads to a quantity known as fluorescence yield which is defined as the product of fluorophore concentration and the molecular quantum yield. If a series of measurements of fluorescence yield are performed for different concentrations of one of the fluorophores then equality of the measured fluorescence yields implies the relationship [N.sub.s1][[phi].sub.s1] = [N.sub.2][[phi].sub.2]. (4b) The equality of the measured fluorescence yields would be instrument independent. All instruments that measure the ratio of fluorescence radiance and molecular absorptivity would give the same response for solutions having identical fluorescence yields (Eq. (4b)]. The equality would be true even if the absorption and emission spectra are very different for the two fluorophores. A practical procedure for converting a comparison of fluorescence radiance into a comparison of fluorescence yields is to work with the same fluorophore in the standard solution and in the analyte so that the molecular absorptivities are reasonably matched and cancel out Verb 1. cancel out - wipe out the effect of something; "The new tax effectively cancels out my raise"; "The `A' will cancel out the `C' on your record" wipe out from the comparison of fluorescence radiances. The equality of fluorescence radiance is then equivalent to equality of fluorescence yield, [Eq. (4b)]. An alternative approach would be to design fluorophore whose molecular absorptivity did not depend on wavelength or solvent, e.g., some nanocrystals. Suppose we compare the fluorescence yield of two solutions or suspensions. If the fluorescence yield is the same for the two solutions and if the concentration of fluorophore is known for the two solutions we say that the fluorescence yield of [N.sub.1] molecules of fluorophore s1 per [m.sub.3] is equivalent to the fluorescence yield of [N.sub.2] molecules of fluorophore s2 per [m.sup.3]. This equivalency equivalency the combining power of an electrolyte. See also equivalent. is based on the equality of solution properties (fluorescence yield) and does not depend on the instrument. The equivalency gives a measure of the number of fluorophores in one solution (analyte) relative to a number of fluorophores in another solution (reference); this is the basis for the assignment of MESF value. 3. Assignment of MESF Value to Microbeads In the following, we will describe the procedure for assigning a MESF value to a microbead with immobilized fluorophores. We will equate the fluorescence yield of the microbead suspension to the reference solution. In what follows we assume that the reference solution and the microbeads have the same fluorophore and that the molecular absorptivity is the same for the two. The solution and suspension are prepared with known number concentration of soluble fluorophores, [N.sub.so1], and number concentration of microbeads, [N.sub.b]. Since we assume that fluorescein in both environments has the same molecular absorptivity, the equality of fluorescence radiance is equivalent to equality of fluorescence yields. [N.sub.so1][[phi].sub.so1] = [N.sub.b][[phi].sub.b]. (5a) Using the reference solution as the unit of fluorescence yield we can assign a value of MESF to the microbead as MESF = ([N.sub.A]/1000)[N.sub.so1]/[N.sub.b] (5b) The factor [N.sub.A]/1000 converts number concentration into a molar concentration Noun 1. molar concentration - concentration measured by the number of moles of solute per liter of solution molarity, M concentration - the strength of a solution; number of molecules of a substance in a given volume , [N.sub.A] is the Avogadro constant The Avogadro constant (symbols: L, NA), also called the Avogadro number is the number of "entities" (usually, atoms or molecules) in one mole,[1][2] that is the number of carbon-12 atoms in 12 grams (0. , and 1000 is the number of [cm.sup.3] in a liter (we use [cm.sup.3] to conform to Verb 1. conform to - satisfy a condition or restriction; "Does this paper meet the requirements for the degree?" fit, meet coordinate - be co-ordinated; "These activities coordinate well" laboratory practice). An example of the above procedure is shown in Fig. 3 where the two arrows show a graphical display of the equivalence of fluores cence yield from a microbead suspension (horizontal arrow) and the concentration of the reference solution, [N.sub.sol] = [N.sub.eq] (mol/L), which gives an equal fluorescence yield. The fluorescence yield of the solution is obtained from a straight line fitted to measured fluorescence yield of six serial dilutions of the reference solution. The number concentration of microbeads was measured using a Coulter particle counter A particle counter is an instrument that detects and counts particles. Applications of particle counters are separated into two primary categories:
intr.v. fluo·resced, fluo·resc·ing, fluo·resc·es To undergo, produce, or show fluorescence. [Back-formation from fluorescence. nce yield as the fluorophores immobilized on a single microbead. The MESF value accounts for the change in quantum yield between fluorophores in solution and immobilized on the microbead. The procedure for assigning MESF values to microbeads requires accurate measurement of the particle concentration and emission spectra. The particle concentration can be obtained using a Coulter particle counter. The emission spectra are difficult to measure for the microbeads with low number of immobilized particles. Scattering can be eliminated by using two holographic See holographic storage. notch filters in the apparatus (Fig. 1). The background contribution from the buffer solution has to be subtracted with care (a buffer solution has several constituents in order to maintain a constant pH). The emitted (fluorescence) photons can also scatter from the microbeads in solution and thus either increase or decrease the observed fluorescence intensity. The biases due to fluorescence scattering have to be investigated. Performing the measurements on a set of reference solutions and a set of microbeads with different number of immobilized fluorophore, we obtain a set of microbeads with different values of MESF. These microbeads can be used to calibrate To adjust or bring into balance. Scanners, CRTs and similar peripherals may require periodic adjustment. Unlike digital devices, the electronic components within these analog devices may change from their original specification. See color calibration and tweak. the response of a flow cytometer. 4. Application of MESF Units The assignment of MESF values to the microbeads is independent of the spectral properties of the fluorophores in reference solution and on the microbead. This was ensured by integrating over the entire corrected emission spectrum [see Appendix Eqs. (16A) and (17A)]. However, when microbeads are applied to calibrating a cytometer, the measuring instrument may sample over a limited range of emission wavelengths. Furthermore the instrument response will usually not be corrected for spectral response. The signal, [S.sub.f]([[lambda].sub.0]), of an instrument (photomultiplier tube A vacuum tube that converts light into electrical energy and amplifies it. Photomultiplier tubes are used in high-end drum scanners, because they are more sensitive to light than the CCD elements used in lower-cost devices. or CCD) can be modeled using Eq. (A12) in the Appendix: [S.sub.f]([[lambda].sub.0]) = [L.sub.f]([[lambda].sub.0]) [GAMMA] R([[lambda].sub.0] [DELTA][[lambda].sub.m]. (6) [L.sub.f]([[lambda].sub.0]) is the spectral radiance of the source, and [DELTA][[lambda].sub.m] is the bandwidth of the emission, [GAMMA] is the throughput of the detection system and the function R ([lambda]) describes the responsivity of the detection system. To be specific, we assume that the instrument is a flow cytometer so that N represents the number of fluorophores on the particle passing the detection region. In order to quantify the response of a biological cell we find a microbead such that the fluorescence signals of the cell and the microbead are equal. The equality of the two signals is modeled by the following equation derived from Eqs. (2) and (6): [N.sub.C][[epsilon].sub.ex,C][[phi].sub.C][integral]R([lambda][S.sub. c]([lambda])d[lambda] = [N.sub.b][[epsilon].sub.ex,b][[phi].sub.b][integral]R([lambda][S.sub. b]([lambda]d[lambda]. (7) The function s([lambda]) is the relative spectral emission, and the subscripts C and b stand for biological cell and calibrated cal·i·brate tr.v. cal·i·brat·ed, cal·i·brat·ing, cal·i·brates 1. To check, adjust, or determine by comparison with a standard (the graduations of a quantitative measuring instrument): microbead, respectively. The above equation models the situation where the cell and the microbead give the same response on the instrument. The equality of the two fluorescence signals is used to assign the same MESF value to the cell as the microbead. Equation (7) points to the fact that the assigned MESF value depends on the properties of the instrument's detection system, R. This could lead to problems since the assigned values of MESF would be instrument dependent. The instrument factor drops out of Eq. (7) if the fluorophores on the analyte and microbead have the same spectral functions s([lambda]). Furthermore if the fluorophores on the analyte and microbead have the same extinction coefficient, Eq. (7) reduces to a equality of fluorescence yields (products of fluorophore number and quantum yield). [N.sub.C][[phi].sub.C] = [N.sub.b][[phi].sub.b]. (8) The biological cell has an assigned value of MESF which is the same as that of the microbead because both have the same fluorescence yield. However, the actual number of fluorophores may not be the same on the two objects. In practice, the buffer (for biological cells and microbeads) that is used in a cytometer measurement is different from the buffer (for microbeads and the Standard Reference Material, SRM) that is used in the assignment of MESF values to the microbeads Eq. (5a). In order that the assignment of MESF value to the microbead be independent of the buffer used, the quantum yields in Eq. (5a) have to change proportionately in different buffers. This is an important assumption underlying the utility of MESE MESE. An ancient word used to signify house, probably from the French maison; it is said that by this word the buildings, curtilage, orchards and gardens will pass. Co. Litt. 56. concept. However if the microbead MESF assignment is independent of the buffer, then Eq. (8) provides a valid transfer of the microbead MESF value to the biological cell. In summary, we restate re·state tr.v. re·stat·ed, re·stat·ing, re·states To state again or in a new form. See Synonyms at repeat. re·state that the MESF value is assigned to the biological cell using the criteria that the fluorescence yields are the same for the biological cell and the microbead with which it is compared. The fluorescence yield is equivalent to fluorescence intensity only if molecular absorptivities are the same (the absorption spectra match or have been used to normalize normalize to convert a set of data by, for example, converting them to logarithms or reciprocals so that their previous non-normal distribution is converted to a normal one. the fluorescence intensity). The value of MESF assigned to the biological cell will be independent of the instrument if the microbead and the cell are measured on the same instrument with the same settings, and the emission spectra match. In a subsequent paper we use Eq. (7) to estimate the variation in the assigned MESF values if the microbeads and biological cells have slightly different absorption and emission properties, and if the instruments have different filters. 5. Utility of MESF The fluorescence from biological cells originates from fluorophores conjugated conjugated adj. Conjugate. estrogens, conjugated Warning - Hazardous drug! C.E.S. to antibodies which are bound to receptors (antigen) present on the walls of the biological cell. Using the same procedure that was described for microbeads, it is possible to assign MESF values to antibodies with conjugated fluorophores (labeled antibodies). It is a good assumption that the value of MESF assigned to the labeled antibodies does not change appreciably when the antibodies are bound to cells. Thus the value of MESF assigned to the entire cell in a flow cytometer can be equated to the product of MESF of the individual labeled antibodies and the number of antibodies on the cell. Dividing the value of the MESF assigned to the cell by the MESF of a single antibody would yield the actual number of antibodies on the biological cell which is the number of interest to the biologist. It is important to note that the number of antibodies bound to the surface of the biological cell is not necessarily equivalent to the number of receptor (antigen) molecules expressed on the biological cell (antigen density). The relationship between the amount of bound antibody and the amount of receptors (antigen) on the biological cell is complicated by many factors, and therefore careful experiments are required to reach an accurate assessment of that relationship. 6. Conclusion We developed a conceptual framework For the concept in aesthetics and art criticism, see . A conceptual framework is used in research to outline possible courses of action or to present a preferred approach to a system analysis project. for interpreting fluorescence radiance measurements and introduced the notion of fluorescence yield which is the measure fluorescence radiance divided by the molecular absorptivity. We then showed that the equivalence of fluorescence yields of two solutions leads to the notion of equivalent number of fluorophores in the two solutions. This is the basis for assigning a MESF value for one solution or suspension in terms of a reference solution. The concepts were applied to quantitating flow cytometer measurements by the following procedure. First, MESF values are assigned to the microbeads with immobilized fluorophores using a standard reference solution. Second, a cytometer is used to compare the fluorescence intensity of microbeads and biological cells with bound labeled antibodies. Equality of fluorescence intensity is then used to determine MESF values of the biological cells. MESF is a stoichiometric stoi·chi·om·e·try n. 1. Calculation of the quantities of reactants and products in a chemical reaction. 2. The quantitative relationship between reactants and products in a chemical reaction. unit for the fluorescence intensity of labeled particles or cells expr essed as the number of fluorophore molecules in solution required to produce the same fluorescence yield as that measured on the labeled particles or cells. For example, if a cell labeled with fluorescein emits as much fluorescence as 5000 molecules of fluorescein in solution, it is assigned a value of 5000 MESF. However, this does not mean that the cell is labeled with 5000 fluorescein molecules, but rather with enough molecules of fluorescein to have the same level of emission as 5000 molecules of fluorescein in solution under similar conditions. The procedure used for cytometers could be modified and extended to quantitating fluorescence intensity measurements in DNA microarray DNA microarray A small solid support, usually a membrane or glass slide, on which sequences of DNA are fixed in an orderly arrangement. DNA microarrays are used for rapid surveys of the expression of many genes simultaneously, as the sequences contained on a . 7. Appendix A. Derivation derivation, in grammar: see inflection. of the Measurement Equation The experimental setup, execution, and analysis of measurements involving optical radiation are greatly simplified by using a measurement equation. This equation mathematically describes the measurement, relating the signal from the detector to the optical properties of the incident light, sample, and detection system. The measurement equation for the total fluorescent radiance is derived in this Appendix in a four-step process. In the first three steps equations are derived for the fluorescence radiant flux radiant flux n. The rate of flow of radiant energy. Noun 1. radiant flux - the rate of flow of radiant energy (electromagnetic waves) flux - the rate of flow of energy or particles across a given surface , the signal from the detection system, and the fluorescent spectral radiance. The last step combines all of the concepts into a measurement model for fluorescence radiance. Much of the derivation is based upon concepts presented by K. D. Mielenz, "Photoluminescence Spectrometry spectrometry /spec·trom·e·try/ (spek-trom´e-tre) determination of the wavelengths or frequencies of the lines in a spectrum. spec·trom·e·try n. " in Optical Radiation Measurements, Volume 3, Measurement of Photoluminescence, ed., K. D. Mielenz, Academic Press (1982) pp. 2-87. 7.1 Fluorescence Radiant Flux Any measurement of optical radiation involves spectral fluxes
Spectral flux over finite spectral bandwidths. In the case of fluorescence, fluxes of both excitation and emission are present. These are denoted by subscripts x and m, respectively. The radiant flux absorbed by a sample, whether it is fluorescent or not, is given by [[PHI].sub.a]([[lambda].sub.x])[DELTA][[lambda].sub.x] = [[PHI].sub.i]([[lambda].sub.x])[DELTA][[lambda].sub.x](1 - [10.sup.-[epsilon]([[lambda].sub.x])NI]), (A1) where [[lambda].sub.x] (nm) and [DELTA](nm) are the wavelength and spectral bandwidth of the excitation radiant flux, respectively, [[PHI].sub.a] (W/nm) and [[PHI].sub.i] (W/nm) are the absorbed and incident spectral fluxes, respectively, [epsilon] ([cm.sup.2]) is the absorptivity, N (1/[cm.sup.3]) is the concentration of fluorophore, and l (cm) is the path length. Expanding the expression in parentheses See parenthesis. parentheses - See left parenthesis, right parenthesis. and keeping only the first-order term, Eq. (A1) becomes [[PHI].sub.a]([[lambda].sub.x])[DELTA][[lambda].sub.x] = 2.3Nl[epsilon]([[lambda].sub.x])[[PHI].sub.i]([[lambda].sub.x])[DELTA ] [[lambda].sub.x]. (A2) The radiant flux from fluorescence is a fraction of the excitation radiant flux, and is given by [[PHI].sub.f]([[lambda].sub.m],[[lambda].sub.x])[DELTA] = y([[lambda].sub.m],[[lambda].sub.x])[DELTA] [[lambda].sub.m][[PHI].sub.a]([[lambda].sub.x])[DELTA][[lambda].sub.x ], (3) where [[lambda].sub.m] (nm) and [DELTA][[lambda].sub.m] (nm) are the wavelength and spectral bandwidth of the emission radiant flux, respectively, [[PHI].sub.f] (W/nm) is the fluorescent spectral flux, and y (1/nm) is the spectral quantum yield. Note the y relates the absorbed radiant flux at wavelength [[lambda].sub.x] to the fluorescent radiant flux at wavelength [[lambda].sub.m]. Using the expression for the absorbed radiant flux from Eq. (A2), Eq. (A3) becomes [[PHI].sub.f]([[lambda].sub.m],[[lambda].sub.x])[DELTA][[lambda].sub. m] = 2.3Nly([[lambda].sub.m],[[lambda].sub.x])[DELTA][[lambda].sub.m][epsi lon]([[lambda].sub.x])[DELTA][[lambda].sub.x]. (A4) 7.2 Relation Between Detector Signal and Source Spectral Radiance Figure 4 shows a schematic diagram of an aperture system for a measurement system consisting of a wavelength selector (programming) selector - 1. In Smalltalk or Objective C, the syntax of a message which selects a particular method in the target object. 2. An operation that returns the state of an object but does not alter that state. and an optical detector (not shown in Fig. 4), be it a filter and detector, a monochromator and a single detector, or a monochromator and an array detector. The signal at a given wavelength setting of the detection system is given by S([[lambda].sub.0]) = [integral][[PHI].sub.D]([[lambda].sub.m])R([[lambda].sub.m])R([[lambd a].sub.0],[[lambda].sub.m])d[[lambda].sub.m]. (A5) Here, [[lambda].sub.0] (nm) is the wavelength setting of the detection system, S (A) is the signal, [[PHI].sub.D] (W/nm) is the spectral flux entering the detector, R (A/W A/W Awaiting A/W Alloy Wheels A/W A-Wing (Star Wars) A/W Actual Weight A/W Alternate Weeks A/W Automatic Win (gaming) ) is the responsivity whose dependence on both [[lambda].sub.0] and [[lambda].sub.m] is shown explicitly, and [[lambda].sub.m] (nm) is the wavelength of the emission radiant flux. For any wavelength selector with a narrow spectral bandwidth, such as an monochromator, R([[lambda].sub.0], [[lambda].sub.m]) is a sharply peaked function about [[lambda].sub.0], in which case Eq. (A5) becomes S([[lambda].sub.0]) = [[PHI].sub.D]([[lambda].sub.0])R([[lambda].sub.0])[DELTA][[lambda].su b.m], (A6) The spectral flux entering the detector is related to the spectral radiance of the source by [[PHI].sub.D]([lambda].sub.0]) = L([[lambda].sub.0]) [GAMMA] = L([[lambda].sub.0]) [A.sub.E][A.sub.s]/[D.sup.2], (A7) where L[W/([m.sup.2] nm sr)] is the spectral radiance, [A.sub.E] ([m.sup.2]) is the area of the entrance aperture of the collection optics, [A.sub.s] ([m.sup.2]) is the area of the image of the entrance slit in the source plane, D ([m.sup.2]) is the distance between the entrance aperture and the source plane, and I ([m.sup.2] sr) is defined by Eq. (A7). Using Eq. (A7), Eq. (A6) becomes S([[lambda].sub.0]) = L([[lambda].sub.0])[GAMMA]R([[lambda].sub.0])[DELTA][[lambda].sub.m], (A8) 7.3 Fluorescent Spectral Radiance The fluorescence source in a cuvette measurement is a volume source with dimensions set by the illuminating beam. Radiance standards are surface sources with known radiance per unit area of the surface. To compare the fluorescence source to the standard source we need to convert the volume source into an equivalent surface source. The spectral radiance from fluorescence source can be defined in terms of the spectral flux from fluorescence. Eq (A4), as [L.sub.f]([[lambda].sub.m], [[lambda].sub.x]) [DELTA][[lambda].sub.m] = f/4[pi] 1/[n.sub.s][A.sub.B] [[PHI].sub.f]([[lambda].sub.m], [[lambda].sub.x])[DELTA] [[lambda].sub.m] = F[[PHI].sub.f]([[lambda].sub.m], [[lambda].sub.x])[DELTA][[lambda].sub.m], (A9) [A.sub.B] ([m.sup.2]) is the cross section area of the intersection between the cylindrical cyl·in·dri·cal adj. Of, relating to, or having the shape of a cylinder, especially of a circular cylinder. volume illuminated by the incident laser beam and the source plane (see Fig. 4.) The factor 4[pi] is the total steridians into which the fluorescence is emitted and f is a angle-dependent function which describes possible non-isotropic emission. The solution index of refraction Index of refraction A constant number for any material for any given color of light that is an indicator of the degree of the bending of the light caused by that material. Mentioned in: Eye Glasses and Contact Lenses , [n.sub.s], corrects for distortion due to refraction refraction, in physics, deflection of a wave on passing obliquely from one transparent medium into a second medium in which its speed is different, as the passage of a light ray from air into glass. at the cuvette boundary. The factor F (1/[m.sup.2]sr) as defined in Eq. (9A), converts the total fluorescence radiant flux (W/nm) into fluorescence spectral radiance [W/nm [m.sup.2] sr)]. The conversion permits us to compare the fluorescence spectral radiance to standard sources whose properties are always defined in terms of spectral radiance. Using Eq. (A4), Eq. (A9) becomes [L.sub.f]([[lambda].sub.m], [[lambda].sub.x])[DELTA][[lambda].sub.m] = 2.3Fnly([[lambda].sub.m], [[lambda].sub.x])[DELTA][[lambda].sub.m] [epsilon]([[lambda].sub.x])[[PHI].sub.i] ([[lambda].sub.x])[DELTA][[lambda].sub.x], (A10) 7.4 Measurement of the Fluorescent Radiance The responsivity of the detection system is calibrated by a source of known spectral radiance L'([[lambda].sub.0]) [W/([m.sup.2] nm sr)]. This source can be either an integrating sphere with known spectral radiance at its exit port or a diffuse reflector reflector: see telescope. , of known reflectance re·flec·tance n. The ratio of the total amount of radiation, as of light, reflected by a surface to the total amount of radiation incident on the surface. Noun 1. factor, illuminated by a source of known spectral irradiance ir·ra·di·ant adj. Sending forth radiant light. [Latin irradi . The emitting surface of the standard source coincides with the source plane in Fig. 4. Using Eq. (A8), the signal S'([[lambda].sub.0]) resulting from the source of known spectral radiance is S'([[lambda].sub.0]) = L'([[lambda].sub.0][GAMMA]R([[lambda].sub.0])[DELTA][[lambda].sub.m], (A11) Likewise, the signal [S.sub.f]([[lambda].sub.0]) resulting from the fluorescent source is [S.sub.f]([[lambda].sub.0]) = [L.sub.f]([[lambda].sub.0])[GAMMA] R([[lambda].sub.0])[DELTA][[lambda].sub.m], (A12) Taking the ratio of Eqs. (A11) and (A12) and using the expression for the fluorescent spectral radiance from Eq. (A10) yields [L.sub.f]([[lambda].sub.0] = [S.sub.f]([[lambda].sub.0])/S'([[lambda].sub.0] L'([[lambda].sub.0]) = 2.3Fnly([[lambda].sub.m], [[lambda].sub.x])[epsilon]([[lambda].sub.x])[[PHI].sub.i]([[lambda].s ub.x])[DELTA][[lambda].sub.x], (A13) Equation (A13) expresses the measured fluorescent spectral radiance [L.sub.f] at a given wavelength setting of the detection system [[lambda].sub.0] both in terms of measured or known quantities ([S.sub.f], S', and L') and in terms of properties of the instrument (F, l, [[PHI].sub.i]([[lambda].sub.x]), and [DELTA][[lambda].sub.x]) and the sample (N, y, and [epsilon]). The spectral quantum yield y([[lambda].sub.m], [[lambda].sub.x]) is conveniently separated into a quantum yield [PHI] and a relative spectral emission function s([[lambda].sub.m], [[lambda].sub.x]) (1/nm), where [integral]s ([[lambda].sub.m], [[lambda].sub.x])d[[lambda].sub.m] = 1. (A14) The total fluorescent radiance [L.sub.f] [W/([m.sup.2] sr)] is given by [L.sub.f] = [integral][L.sub.f]([[lambda].sub.0])d[[lambda].sub.0]. (A15) Substituting the right-hand expression in Eq. (A13) for [L.sub.f]([[lambda].sub.0]) in Eq. (15) and using Eq. (A14) yields the measurement equation relating the total fluorescent radiance to the appropriate instrument and sample properties, namely [L.sub.f] = 2.3 FNl[phi][epsilon]([[lambda].sub.x])[[PHI].sub.i]( [[lambda].sub.x])[delta] [[lambda].sub.x]. (A16) In terms of measured and known quantities, the total fluorescent radiance, again using Eqs. (A 15) and (A 13), is [FORMULA NOT REPRODUCIBLE IN ASCII ASCII or American Standard Code for Information Interchange, a set of codes used to represent letters, numbers, a few symbols, and control characters. Originally designed for teletype operations, it has found wide application in computers. ] (A17) Equations (A 16) and (A 17) constitute the measurement model of fluorecence radiance. The measured fluorescence radiance [Eq. (A 17)] is equated to the fluorescence radiance which results from known solution and measurement properties. [FIGURE 1 OMITTED] [FIGURE 2 OMITTED] [FIGURE 3 OMITTED] Accepted: November 29, 2001 8. References (1.) J. R. Lakowicz, Principles of Fluorescence Spectroscopy Fluorescence spectroscopy or fluorometry or spectrofluorimetry is a type of electromagnetic spectroscopy which analyzes fluorescence from a sample. It involves using a beam of light, usually ultraviolet light, that excites the electrons in molecules of certain , Kluwer Academic/Plenum Publishers, New York New York, state, United States New York, Middle Atlantic state of the United States. It is bordered by Vermont, Massachusetts, Connecticut, and the Atlantic Ocean (E), New Jersey and Pennsylvania (S), Lakes Erie and Ontario and the Canadian province of (1999). (2.) G. T. Hermanson, Bioconjugate Techniques, Academic Press, Inc., San Diego San Diego (săn dēā`gō), city (1990 pop. 1,110,549), seat of San Diego co., S Calif., on San Diego Bay; inc. 1850. San Diego includes the unincorporated communities of La Jolla and Spring Valley. Coronado is across the bay. (1996). (3.) P. B. Fernandes, Technological Advances in High-Throughput Screening High-throughput screening (HTS), is a method for scientific experimentation especially used in drug discovery and relevant to the fields of biology and chemistry. Purpose and method , Curr. Opin. Chem. Biol. 2, 597-603 (1998). (4.) S. Weiss, Measuring Conformational Dynamics of Biomolecules This page aims to list articles on Wikipedia that describe particular biomolecules or types of biomolecules. This list is not necessarily complete or up to date - if you see an article that should be here but isn't (or one that shouldn't be here but is), please update the page by Single Molecule Fluorescence Spectroscopy, Nat. Struct. Biol. 7, 724-729 (2000). (5.) J. W. Gratama, J.-L. D'hautcourt, F. Mandy, G. Rothe, D. Barnett, G. Janossy, S. Papa, G. Schmitz, and R. Lenkei, Flow Cytometric Quantitation of Immunofluorescence Immunofluorescence A technique that uses a fluorochrome to indicate the occurrence of a specific antigen-antibody reaction. The fluorochrome labels either an antigen or an antibody. Intensity: Problems and Perspectives, Cytometry 33, 166-178 (1998). (6.) R. F. Vogt, G. D. Cross, D. L. Phillips, L. O. Henderson, and W. H. Hannon, Interlaboratory Study of Cellular Fluorescence Intensity Measurements with Fluorescein-Labeled Microbead Standards, Cytometry 12, 525-536 (1991). (7.) A. Schwartz, E. F. Repollet, R. Vogt, and J. W. Gratama, Standardizing Flow Cytometry flow cytometry (flōˑ sī·t  ˑ·m : Construction of a Standardized Fluorescence Calibration Plot Using Matching Spectral Calibrators, Cytometry 26, 22-31 (1996). (8.) R. Sjoback, J. Nygren, and M. Kubista, Absorption and fluorescence properties of fluorescein, Spectrochimica Acta Part A 51, L1-L21 (1995). (9.) N. Klonis and W. H. Sawyer, Spectral Properties of the Prototropic Forms of Fluorescein in Aqueous aqueous /aque·ous/ (a´kwe-us) 1. watery; prepared with water. 2. see under humor. a·que·ous adj. Solution, J. Fluorese. 6, 147-157 (1996). (10.) N. Periasamy, S. Bicknese, and A. S. Vcrkman, Reversible Photobleaching Photobleaching is the photochemical destruction of a fluorophore. In microscopy, photobleaching may complicate the observation of fluorescent molecules, since they will eventually be destroyed by the light exposure necessary to stimulate them into fluorescing. of Fluorescein Conjugates in Air-saturated Viscous viscous /vis·cous/ (vis´kus) sticky or gummy; having a high degree of viscosity. vis·cous adj. 1. Having relatively high resistance to flow. 2. Viscid. Solutions: Singlet and Triplet triplet /trip·let/ (trip´let) 1. one of three offspring produced at one birth. 2. a combination of three objects or entities acting together, as three lenses or three nucleotides. 3. State Quenching quenching Rapid cooling, as by immersion in oil or water, of a metal object from the high temperature at which it is shaped. Quenching is usually done to maintain mechanical properties that would be lost with slow cooling. by Tryptophan tryptophan (trĭp`təfăn), organic compound, one of the 20 amino acids commonly found in animal proteins. Only the l-stereoisomer appears in mammalian protein. , Photochem. Photobiol. 63, 265-271 (1996). (11.) R. Sjoback, J. Nygren, and M. Kubista, Characterization of Fluorescein-Oligonucleotide Conjugates and Measurement of Local Electrostatic Stationary electrical charges in which no current flows. For example, laser printers and copier machines place a positive charge of the image on a drum, and negatively charged toner is attracted onto the drum. The toner is then transferred to positively charged paper and fused to the paper by heat. Potential, Biopolymers 46, 445-453 (1998). About the Authors: Abe Schwartz
Abe Schwartz (1881-1963) was a well-known klezmer musician of the 1920s. Abe was born outside of Bucharest, Romania, and moved to the United States in 1899. is a chemist at the Center for Quantitative Cytometry. Lili Wang Lili Wang (March 6 1971 - October 12 2002) was a graduate student at North Carolina State University murdered by another graduate student named Richard Anderson. On that day, Anderson shot and killed her while she was playing tennis. is a guest scientist and A. Gaigalas is a physicist both in the Biotechnology Division of the NIST (National Institute of Standards & Technology, Washington, DC, www.nist.gov) The standards-defining agency of the U.S. government, formerly the National Bureau of Standards. It is one of three agencies that fall under the Technology Administration (www.technology. Chemical Science and Technology Laboratory. E. Early is a physicist in the Optical Technology Division of the NIST Physics Laboratory. Yu-zhong Zhang is a biochemist at Molecular Probes Molecular Probes is a biotechnology company located in Eugene, Oregon specializing in fluorescence. The company was founded in 1975 by Richard and Rosaria Haugland in their kitchen in Minnesota, then moved briefly to Texas and finally to Oregon in the early 1980s. , Inc. G. E. Marti is a review and research officer at CBER CB·er n. One that uses a CB radio. , FDA FDA abbr. Food and Drug Administration FDA, n.pr See Food and Drug Administration. FDA, n.pr the abbreviation for the Food and Drug Administration. and an attending physician at the NCI See Liberate. . R. F. Vogt is a chemist at the Center of Disease Control and Prevention, Atlanta, GA. The National Institute of Standards and Technology National Institute of Standards and Technology, governmental agency within the U.S. Dept. of Commerce with the mission of "working with industry to develop and apply technology, measurements, and standards" in the national interest. is an agency of the Technology Administration, U.S. Department of Commerce. |
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