AU618016B2 - Device and method for the determination of incisional wound healing ability - Google Patents

Device and method for the determination of incisional wound healing ability Download PDF

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Publication number
AU618016B2
AU618016B2 AU20886/88A AU2088688A AU618016B2 AU 618016 B2 AU618016 B2 AU 618016B2 AU 20886/88 A AU20886/88 A AU 20886/88A AU 2088688 A AU2088688 A AU 2088688A AU 618016 B2 AU618016 B2 AU 618016B2
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Australia
Prior art keywords
wound
sponge
capillary tube
healing
cells
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AU20886/88A
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AU2088688A (en
Inventor
Rainer Govenius
Timo Hurula
Kurt Lonnqvist
Jouko Viljanto
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Huhtamaki Oyj
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Huhtamaki Yhtyma OY
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Priority claimed from FI873075A external-priority patent/FI77569C/en
Application filed by Huhtamaki Yhtyma OY filed Critical Huhtamaki Yhtyma OY
Publication of AU2088688A publication Critical patent/AU2088688A/en
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    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61BDIAGNOSIS; SURGERY; IDENTIFICATION
    • A61B10/00Other methods or instruments for diagnosis, e.g. instruments for taking a cell sample, for biopsy, for vaccination diagnosis; Sex determination; Ovulation-period determination; Throat striking implements
    • A61B10/02Instruments for taking cell samples or for biopsy

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  • Health & Medical Sciences (AREA)
  • Life Sciences & Earth Sciences (AREA)
  • Medical Informatics (AREA)
  • Engineering & Computer Science (AREA)
  • Biomedical Technology (AREA)
  • Heart & Thoracic Surgery (AREA)
  • Pathology (AREA)
  • Molecular Biology (AREA)
  • Surgery (AREA)
  • Animal Behavior & Ethology (AREA)
  • General Health & Medical Sciences (AREA)
  • Public Health (AREA)
  • Veterinary Medicine (AREA)
  • Investigating Or Analysing Biological Materials (AREA)

Description

F AU-AI-20886/ 8 8 WORLD INTELLECTUAL PROPERTY ORGANIZATION International Bureau
PCT
INTERNATIONAL APPLICATION PUBLISHED UNDER THE PATENT COOPERATION TREATY (PCT) (51) International Patent Classification 4 (11) International Publication Number: WO 89/ 00403 A61B 10/00 Al (43) Interna'hal4kblic n at: 2an t 1989 (26.01.89) (21) Internaiional Application Number: PCT/FI88/00113 74 Agent: LEITZINGER OY; Hietalaildenkatu a A, SF- 00180 Helsinki (FI).
(22) International Filing Date: 8 July 1988 (08.07.88) (81) Designated States: AT (European patent), AU, BE (Eu- (31) Priority Application Number: 873075 ropean patent), BG, BJ (OAPI patent), BR, CF (OA- PI patent), CG (OAPI patent), CH (European pa- (32) Priority Date: 13 July 1987 (13.07.87) tent), CM (OAPI patent), DE (European patent), DK, FR (European patent), GA (OAPI patent), GB (Euro- (33) Priority Country: FI pean patent), HU, IT (European patent), JP, KP, KR, LU (European patent), ML (OAPI patent), MR (OA- PI patent), NL (European patent), NO, RO, SE (Eu- (71) Applicant (for all designated States except US): HUH- ropean patent), SN (OAPI patent), SU, TD (OAPI TAMAKI OY [FI/FI]; Kirsamaentie 35, SF-20100. patent), TG (OAPI patent), US.
Turku (FI).
(72) Inventors; and Published Inventors/Applicants (for US only) VILJANTO, Jouko With international search report.
[FI/FI]; Terhokatu 18, SF-20720 Turku GOVE- NIUS, Rainer..[FI/FI]; Eristajanmutka 29, SF-20310 Turku LONNQVIST, Kurt [FI/FI]; Uudenma- AUSTRALIAN ankatu 12 B, SF-20500 Turku HURULA, TimoLI [FI/FI]; Tuureporinkatu 14 B 31, SF-20110 Turku FEB 1989 TN OFFIC PATENT
OFFICE
(54)Title: DEVICE AND METHOD FOR THE DETERMINATION OF [NCISIONAL WOUND
TY
HEALING ABILI- =Now.: _71" 7 7~ (57) Abstract The object of the invention is a device for determining the healing ability of a surgical wound or a connective tissue.
A flexible capillary tube is inserted into the wound, the said tube having at the end to be inserted a sponge for the attachment and growth of cells. At least that end of the capillary tube which is left inside the wound is provided with at least one inner groove. The sponge is a wet-expanding viscose cellulose sponge containing macro- and micropores in communication with each other.
i WO 89/00403 Device and method f wound healing abili The present inven-z PCT/F188/00113 or the determination of incisional ty on _lar-es to a device and a method for the determination of the healing ability of an incisional wound or a connective tissue in man.
The tissue healing process begins within a matter of seconds from receiving a lesion or starting an operation and continues via blood coagulation and a highly diversified biological reaction chain towards connective tissue cicatrization. What in the beginning is a cell-abundant, slack and mechanically unstable tissue turns into a firmer and firmer tissue as days and weeks pass. Little by little the metabolism of this granulation tissue becomes slower. The shape, final size and microscopic texture of a cicatrix tissue are determined according to the patient's age, sex, general metabolism and local tissue strength requirement.
With animal experiments it has been possible to indicate that the amount of cells appearing in the wound area during the first days and the relative quantitative proportions thereof determine the course of healing for weeks onwards.- Although it is possible with test animals to study the local healing rate of tissues in many different ways from the wound itself, this has not been possible with human beings. Clinically estimated, the healing of tissues is either a success or a failure.
No information has been obtainable from a closed incisional wound about the deceleration of healing and the reasons possibly contributing to this.
There is a prior known device and method for collecting wound cells from an incisional wound (Viljanto-, J.,
I
d n
D
I I
I
-2- J. Sug. Res. 20 (1979) p. 115-119). In this prior known method a thin silicone rubber tube with a cellulose sponge at one end is placed in the wound for picking up a sample of wound cells for analysis. An object of the present invention is to improve this device and method for providing a reliably operating, tissue-healing testing device as well as a method which is reliably reproducible and whereby the accuracy of analysis results is improved and their utilization is facilitated.
According to the present invention there is provided a device for collecting wound exudate from an incisional wound for examination, said device including a flexible open ended capillary tube to be left inside a wound, the tube I end to be placed in a wound being fitted with a sponge intended for the attachment and growth of cells, wherein at least the end of capillary tube to be left in the wound is provided with at least one inner groove to enable exudate to penetrate into said capillary tube, said sponge being a wet-expanding viscose i cellulose sponge containing "macro"-and "micropores" (as hereinbefore defined) '5 in communication with each other and the distribution mean of micropores is S within the range of 5 to 15pm and the average distribution mean of the diameters of micropores is within the range of 0.4 to 0.9 mm. The inner design of a capillary tube according to the invention provides a firm attachment of the sponge to the end of a tube and at the same time there is secured the free entrance and movement for cell-containing wound exudate in the capillary tube and in the sponge. In a preferred embodiment, the interior of a capillary tube is divided into four substantially equi-sized grooves. This produces two opposite pairs of grooves having therebetween ridges retaining the piece of sponge.
The viscose cellulose sponge is preferably rectangular in cross-section and so dimension that, when dry, it extends from one groove of a capillary tube to the op-
/F
I'?T
wo 89/00403 PCT/F188/00113 posite grdove, the side grooves remaining free even in the expanded condition of a viscose sponge, wherebv z'e fluid is illowed a free flow in the .e free se grooves. The capillary tube is preferably made of silicone rubber.
The invention relates also to a method for the determination of incisional wound healing ability, wherein a sponge mounted on a capillary tube and intended for the attachment and growth of wound cells is inserted in a wound for sampling. This invention is characterized in that, after the sampling, the sponge is rinsed with a certain rinsing liquid, at a certain rinsing speed and with a certain amount of rinsing liquid, followed by treating the cell suspension in a per se known manner for differential counting of the cells and and comparing the obtained reLults with reference values.
Tho comparison is most preferably effected by means of a computer.
With a device of the invention it is possible to obtain already at the early stage of healing, usually after 48 hours, a representative cell specimen anticipating subsequent healing. By means of the further treatment and differential counting of cells it is possible to find out whether the healing of an examined patient's wound is proceeding as would be expected on the basis of his or her age and sex. If there is abnormality in the local cytological response at the early stage of healing, its clinical significance can be clarified in several cases. If the question is about a disturbance caused by the lack of nutrients or trace elements, it can be still be at least partially repaired during the course of healing.
a i i I I i WO 89/00403 PCT/F18/00113 4 It should be appreciated that the analysis of wound cals Ls not solaly intended for anticipating the he-!ing of a wound tested. The cytological response primarily reveals the responsive ability and strength of an examined individual over the entire healing process. It has been said that wound healing is an indicator of the vitality of a whole individual as it requires the coordinated combined effect of all blood cells, connective tissue cells as well as dozens of different enzymes, catalysts and intermediator substances.
In order to make a wound cell analysis reliably reproducible, a device collecting wound cells must be structurally standardized. This is particularly true regarding a cellulose sponge placed inside a slicone rubber tube. Cells are extremely sensitive to even slight changes in the surface texture and pore size of a sponge. Therefore, even microscopically studied, the sponge texture should be homogeneous and dimensionally precisely quantified.
The interpretation of a cellular analysis would not have been practically possible without data processing technology. A method of the invention facilitates the preparation of information obtained from a cellular analysis and suitable for clinical application within a matter of minutes from the moment the data is supplied from a computer terminal. Thereafter, it is possible to collect continuously increasing material for detecting disease-linked and hereditary effects on the healing of tissues.
The invention will now be described in more detail with reference made to the accompanying drawings, in which 1 L WO 89/00403 PCT/F188/00113 fig. 1 shows a device of the invention wrapped in a protective package, fig. 2 shows a device of the invention implanted in a wound, fig. 3 shows the sponge-facing end of a capillary tube as an enlarged longitudinal and crosswise section, fig. 4 shows the same as fig. 3 but the sponge imbibed with fluid, figs. 5 and 6 show the distribution curves for macroand micropores in a prior known sponge and in a sponge of the invention.
A device of the invention comprises a pliable capillary tube 1, which is preferably made of silicone rubber and one end of which is fitted with a wound cells collecting sponge 2. For the purpose of use, this tube 1 of the invention is packed in a transparent protective case 3, in which the capillary tube is fastened to a base sheet by means of protective films. For the puirpose of application, the protective films can be readily torn off from the end of capillary tube 1 and, as shown in fig. 1, a plurality of such capillary packages can be koined side by side and removed one by one.
A capillary tube 1 removed from the package is placed inside a wound as shown in fig. 2. A capillary tube 1 is left in this position for e.g. 48 hours with fluid being collected in capillary tube 1 and absorbed in sponge 2.
m -i r WO 89/00403 PCT/F88/00113 6 It is important that the shape of capillary tube 1 and sponge 2 be such thaz said sponge 2 remains firmi. i position also in an expanded condition. It is also important that wound fluid be able to flow freely in capillary tube 1 and the capillary tube not be blocked by expanded sponge 2. In a solution of the invention (figs. 3 and the capillary tube is provided with at least one inner groove 4, 6. In the case shown in figs. 3 and 4, the number of grooves 4, 6 is four, comprising pairs of grooves 4, 6 disposed in opposite relation to each other. Thus, between the grooves there are formed ridges 5 pointing towards the centre of the tube.
A sponge 2 inserted in the end of tube 1 is rectangular in cross-section and so dimensioned that in a crosssection its opposite ends extend into the corresponding inner grooves 4 of a capillary tube leaving the other pair of inner grooves 6 vacant. In addition, sponge 2 is placed entirely in capillary tube 1 in a manner that, in an expanded condition, said sponge 2 does not extend out of capillary tube 1 (fig. 4) When this capillary tube 1 along with its sponge 2 is placed in a wound, the wound fluid has unhindered entry in capillary tube 1 by virtue of the side grooves 6 on either side of sponge 2. The ridges 5 between grooves 4, 6 prevent viscose sponge 2 from working its way into side grooves 6, which remain vacant and facilitate the flow of wound fluid in the capillary tube.
In order to achieve a preferred result, a viscose sponge 2 used must be as homogeneous as possible.
It must contain both micro- and macropores which are Swo 89/00403 PCT/F188/00113 7 in communication with each other so that wound cells are able to migrate from one pore to another. The sponge must also be clinically clean and so must the capillary tube. In this context, the macropores refer to pores whose diameter is in the order of 1,0 mm and the micropores refer to pores whose diameter or linear measure is in the order of 10 pm. Since the purpose of a sponge is to collect cells from a surgical wound and to offer them a natural culture'medium, its texture is of prime importance in view of the invention and decisive in terms of the function of a viscose sponge. Important in view of the operation is a relative proportion between micro- and macropores, the correct size and shape of pores as well as the openings in the partitions of pores for facilitating the migration of cells from one pore to another.
When studying a human being, it is for practical reasons necessary to employ a small device and, thus, a viscose sponge used is also small. In order to achieve a preferred result, the viscose sponge used must be as homogeneous as possible. A requirement for this is that there will be as little fluctuations as possible in the pore size distribution of a sponge. The peaks of micro- and macropore distributions must be as narrow as possible, especially the presence of a very large macropore in sponge 2 would nullify the entire analysis process.
In the industrially produced sponges, the macropores have been too large in terms of proper functioning by preventing the attachment of cells to the walls of a pore and the macropore distribution has also-been too wide (fig.
I
WO 89/00403 PCT/F188/0013 8 It is important in terms of proper functioning that micropores are as large as possible, distribution mean within the range of 5 15 Pm, and macropores respectively as small as possible, distribution mean within the range of 0,4 0,9 mm (fig. 6).
The manufacturing of a viscose cellulose sponge is known as such. Thus, the manufacturing of a microand macropores containing sponge of the invention proceeds according to prior known methods and can be effected e.g. as follows: In fiber-containing special viscose are added screened sodium sulphate crystals under vacuum. Viscose is solidified and sodium sulphate crystals are removed by dissolving. The sponge is bleached and pressed, dried and cut into pieces of suitable size.
Following the sampling, the outer end of capillary tube 1 is attached to a rinsing device, wherein the sponge is rinsed for recovering the cells collected therein for analysis. In view of the funct:oning and reproducibility of the method it is important to employ a certain rinsing agent, rinsing speed and amount of rinsing liquid. When selecting these parameters, care should also be taken that the cells contained in the sponge do not break during the rinsing operation.
The results obtained in the studies are analyzed and these results are compared with values obtained earlier in similar tests. Due to an extensive and diversified comparison, this can only be practically performed by means of a computer, whereby the result is obtained almost immediately and necessary therapeutical measures can be initiated as quickly as possible.
,i- WO 89/00403 PCT/FI88/00113 9 Clinical use of 6ell sampling device At the end of an operation, prior to the closing of the skin wound, a cellulose sponge cut to a predetermined shape and size and fixed to one end of a silicone rubber tube, is imbibed with 0.9 saline, after which the sampling tube is inserted in the surgical wound in such a way that the open end of the tube is fastened under sterile conditions to the skin with tape.
The sampling tube is removed from the wound after a given time by pulling lightly. The open end of the sampling tube which was on the skin is attached for the rinsing of the sponge to a pump which delivers a constant volume e.g. 2 ml of isotonic citrate solution over a given period, generally 5 seconds. The rinsing liquid, the amount and rate of its supply are selected in such a manner that the cells can be removed from the surface and pores of the sponge without damaging the cells.
After rinsing, sample batches of equal size (200 ul) are taken from the cellular suspension and the samples are centrifuged in a cytocentrifuge at the speed of 1000 rpm for 7 minutes. The cells transferred to slides are air-dried, fixed in absolute ethanol and stained according to the May-Griinwald-Giemsa method in an automatic staining apparatus. From these stained slides is performed a differential count of the cells and the results obtained are compared with the reference material obtained from healthy operated patients.
The healing of the wound is considered normal when the socalled biological healing has progressed as far as the chronological time used for healing requires on a patient of a certain age. If the biological healing, which in this case is measured by the absolute amount of cells in the wound at each point of observation and by the relative proportion of each cell type, has not progressed to the stage required by the WO 89/00403 PCT/F188/00113 chronological healing time, then the healing of the wound has retarded. When biological healing progresses more rapidly than chronological healing, the healing of ;he wound is takin. pace more rapidly than average in the same age group. Using the method for determining the healing speed of a wound requires the existence of comprehensive reference material and its own adpprogram.
Example Let us suppose that the capillary sampling tube is removed 47.8 hours after its insertion into the wound. The chronological time used for healing is thus the same, that is, 47.8 hours. The cell content of the capillary sampling tube, which due to the special structure of this sampling tube corresponds to the type and relative amount of the cells in the surgical wound, is counted subsequent to MGG staining by means of conventional differential counting. The values obtained are fed from the computer terminal to be processed by the CELLCO adp-program and to be compared with the reference material. Each of the ten cell ratios indicates a particular healing time, some ratios more accurately than others. The predicted value of the cell ratios has been taken into account as weighted averages in the adpprogram. Let us suppose that the biological healing time obtained for an example patient is 44.7 hours. The difference between healing times, -3.1 hours, is more than -2SD (-2.4 hours) and thus this difference can be considered significant and the healing of the wound on the example patient slower than average in the same age group. A closer comparison between cell ratios by means of an adp-program into "gates" calculated at 99% confidence limits gives in many cases also suggestive information of the primary reasons for the retardation. In some cases healing can then still be promoted by suitable postoperative treatment.
I~
WO 89/00403 PCT/F188/00113 May it also be pointed out that the cell sample from a wound obtained by means of the sampling tube relating to the invention can, in addition to the foregoing, be studied by means of a variety of biomedical methods in order to solve the special problems relating to the recovery of the patient.
The most common implantation time is 48 hours. Shorter or longer periods can be employed, whereby the rinsing speed of a rinsing liquid changes accordingly. A sampling time of 24 hours requires a slower rinsing speed while a sampling time of 72 hours requires a faster supply speed.

Claims (4)

1. A device for collecting wound exudate from an incisional wound for examination, said device including a flexible open ended capillary tube to be left inside a wound, the tube end to be placed in a wound being fitted with a sponge intended for the attachment and growth of cells, wherein at least the end of capillary tube to be left in the wound is provided with at least one inner groove to enable exudate to penetrate into said capillary tube, said sponge being a wet- expanding viscose cellulose sponge containing "macro"-and "micropores" (as hereinbefore defined) in communication with each other and the distribution mean *i of micropores is within the range of 5 to 15lm and the average distribution mean of the diameters of micropores is within the range of 0.4 to 0.9 mm.
2. The device as set forth in claim 1, wherein said at least one inner groove comprises four substantially equi-sized grooves.
3. The device as set forth in claim 2, wherein said sponge is rectangular S in cross-section and extends in capillary tube from one groove to the opposite groove, thus leaving side grooves vacant also in an expanded condition of the sponge.
4. The device as set forth in any one of claims 1 to 3, wherein said capillary tube is made of oxygen permeable silicone rubber. A device for collecting wound exudate from an incisional wound examination substantially as hereinbefore described with reference to the accompanying drawings. D A T E D this 2nd day of October 1991. +4YS '7lP HUHTAMAKI OY By its Patent Attorneys: CALLINAN LAWRIE ^Jl/Wf^i~
AU20886/88A 1987-07-13 1988-07-08 Device and method for the determination of incisional wound healing ability Ceased AU618016B2 (en)

Applications Claiming Priority (3)

Application Number Priority Date Filing Date Title
FI873075A FI77569C (en) 1987-07-13 1987-07-13 ANORDINATION FOR THE PURPOSE OF THE OPERATIONS AND THE OPERATIONS OF ELLER EN VAEVNAD.
FI873075 1987-07-13
PCT/FI1988/000113 WO1989000403A1 (en) 1987-07-13 1988-07-08 Device and method for the determination of incisional wound healing ability

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AU618016B2 true AU618016B2 (en) 1991-12-12

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Citations (3)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
US3640268A (en) * 1965-10-23 1972-02-08 Hugh J Davis Method and device for biopsy specimen collecting and handling
US3688763A (en) * 1969-07-28 1972-09-05 Raymond Cromarty Diagnostic device and method
US3957054A (en) * 1973-09-26 1976-05-18 Mcfarlane Richard H Surgical drainage tube

Patent Citations (3)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
US3640268A (en) * 1965-10-23 1972-02-08 Hugh J Davis Method and device for biopsy specimen collecting and handling
US3688763A (en) * 1969-07-28 1972-09-05 Raymond Cromarty Diagnostic device and method
US3957054A (en) * 1973-09-26 1976-05-18 Mcfarlane Richard H Surgical drainage tube

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NO900180D0 (en) 1990-01-12
AU2088688A (en) 1989-02-13

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